SERUM/PLASMA MICRONAS AND USES THEREOF
This invention provides a combination of microRNAs for evaluating the physiological and/or pathological condition of a subject, wherein the combination comprises all detectable microRNAs stably existing in the serum/plasma of a subject; and a method for evaluating the physiological and/or pathological condition of a subject, wherein the method includes determining all detectable microRNAs stably existing in the serum/plasma of a subject; and a kit for evaluating the physiological and/or pathological condition of a subject, wherein the kit contains the tools for determining all detectable microRNAs that stably existing in the serum/plasma of a subject; and a biochip for evaluating the physiological and/or pathological condition of a subject, wherein the biochip contains the components for determining all detectable microRNAs stably existing in the serum/plasma of a subject. The aforementioned combination, method, kit and biochip can be used for diagnosis as well as differentially diagnosis of diseases including various tumors; various acute/chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute/chronic infectious diseases caused by various pathogenic microorganisms; other acute/chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular diseases, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system, prediction of complications occurrence and malignant diseases relapse, evaluation of therapeutic effects, screening of pharmaceutical active ingredients, assessment of drug efficacy as well as forensic authentication and prohibited drug inspection and the like, possessing a number of advantages such as extensive detection spectrum, high sensitivity, low cost, convenience for sampling, ease for sample preservation, etc. The said method can be widely used in work related to general survey of diseases and so on, improve the low-specificity and low-sensitivity caused by individual differences which single markers are difficult to overcome, significantly increasing the clinical detection rate of diseases, all of which make it become an effective means for diagnosing diseases in an early phase.
The present invention relates to microRNAs and uses thereof, more specifically, to serum/plasma microRNAs and the uses of serum/plasma microRNAs for diagnosis and differential diagnosis of diseases, prediction of complication occurrence and malignant disease relapse, evaluation of therapeutic effects, screening of pharmaceutical active ingredients, assessment of drug efficacy, forensic authentication and prohibited drug inspection and the like.
BACKGROUND ARTTo locate and precisely detect disease markers has already been the important precondition for the diagnosis and treatment of various clinical diseases including various tumors; various acute/chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute/chronic infectious diseases caused by various pathogenic microorganisms; other acute/chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular diseases, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system. Although more and more disease markers have been found and utilized in general survey and diagnosis of clinical diseases as well as monitoring and controlling of therapeutic effects, their clinical application effects are obviously insufficient. For instance, tumor marker, e.g. alphafetoprotein, lactic dehydrogenase and carcinoembryonic antigen have been widely used in clinic. But these disease markers are far from meeting the needs of early diagnosis for cancer for the following two main reasons: (1) the sensitivity and specificity for the above-mentioned disease markers are relatively low, thus their detection results cannot be used as a diagnostic indicator of disease; (2) the early diagnosis rate of disease shall be positively correlative with the therapeutic effects. However, it is difficult for any of the aforesaid disease markers to meet such requirements for early diagnosis. Take cancer for example, the specificity of tumor differentiation is too high, the integrated sensitivity of tumor is relatively low, the samples sent to be detected are difficult to be repeatedly taken and the conditions to meet the preservation requirements for samples are too exacting, meanwhile, the cost is very high, thus under existing technology the spreading and use of the tumor markers available are hard to realize. The inherent defects of some traditional medical means such as biopsy, for example, incorrect material-extraction position, the inadequacy of sample materials for histocytes and human inexperience, etc., will all lead to misdiagnosis. Although other techniques such as imaging technique have been widely used for examination and diagnosis of diseases, there exists considerable limitation on the determination for disease degree. Consequently, it is very necessary to find out a maker for disease detection which is novel, sensitive and convenient to use and can also overcome the defects of existing markers as mentioned above.
MicroRNAs are defined as a kind of non-coding single-stranded small RNA moleculars of approximately from 19 to 23 nucleotides in length. They are highly conservative in evolution; and are closely related to many normal physiological activities of animals such as development process, tissue differentiation, cell apoptosis and energy metabolism; in addition, bear close relation with the occurrence and development of many diseases. Recent studies show that the expression levels of several microRNAs in chronic lymphocytic leukemia and Burkitt lymphoma are on average down-regulated to various extents; and that by analyzing and comparing the expressions of microRNAs in tissues of human lung cancer and human breast cancer, the expression levels of several tissue specific microRNAs have changed relative to normal tissues. Some studies demonstrate that microRNAs affect the occurrence and development of cardio-cerebrovascular diseases such as myocardial hypertrophy, heart failure, atherosclerosis, and are closely relative to metabolic diseases such as Diabetes II. These experimental results indicate that there exists inevitable connection between the expression and specificity changes of microRNAs and the occurrence and development of diseases.
For the unimaginable important role microRNAs played in the regulation of expression after gene transcription, microRNAs have some associations with diseases. First of all, the changes of microRNAs may be the cause of diseases. This is because both the inhibitor and the promoter of diseases may be target sites for microRNAs. If the expression of microRNA itself is disturbed, e.g., the expression level of microRNA which is originally to inhibit disease promoters decreases or the expression level of microRNA which is to inhibit disease inhibitor increases, its end results will both lead to changes in the expression of downstream genes and the overall disorder of some pathways, further inducing the occurrence of diseases. Secondly, the changes of microRNAs may also result from diseases. This is because, when a kind of disease such as cancer occurs, it will lead to the loss of chromosome segments, gene mutation or rapid amplification of chromosome segments; moreover, if the microRNAs happen to locate in the changing segment, then their expression level will extremely significantly change. Therefore, in theory, microRNAs can be completely regarded as a kind of new disease markers, the specificity changes of which inevitably correlate with the occurrence and development of diseases. Meanwhile, microRNA can also be used as a potential drug target, and it may greatly alleviate the occurrence and development of diseases by inhibiting the up-regulated microRNAs and overexpressedly down-regulated microRNAs in the course of a disease.
The inventor has carried out the research in the relevant fields of using microRNAs as disease markers, for instance, choosing colonic carcinoma which ranks forth in the incidence of malignant tumor as the research object. The research suggests that, during the process of colon benign polyps developing into malignant tumor, some microRNAs exhibit specificity changes, thereby a more sensitive and accurate method for the early diagnosis of colonic carcinoma having been set up through detecting the specific changes in microRNAs. However, since the sampling for tissue specimen is not easy, the wide application of this method in clinics is limited.
DETAILED DESCRIPTION OF THE INVENTIONThe inventor focuses the research on the blood which is relatively easy to obtain and even can be collected via routine physical examination. Blood will circulate to all tissues in body and convey nutrients to cells whilst scavenging waste materials; therefore, blood is able to reflect the physiological pathology of the whole organism and its detection results is an indicator of human health. It is known that in serum/plasma there are many kinds of proteins such as total protein, albumin and globulin, many kinds of lipids such as HDL cholesterol and triglycerides, many kinds of carbohydrates, pigments, electrolytes, inorganic salts, and many kinds of enzymes such as amylase, alkaline phosphatase, acid phosphatase, cholinesterase and aldolase; moreover, there also exist many kinds of signaling molecules such as cytokines and hormone from tissues and organs in whole body. Currently, disease diagnosis is only limited to the above-mentioned biochemical indexes in serum/plasma, and no report is available regarding microRNAs in serum/plasma. It traditionally believed that there is no microRNA in serum/plasma, and that, if any, it will be rapidly degraded by RNase into small molecule segments and hence cannot be detected. However, microRNAs, consisting of from 19 to 23 nucleotides, possess specificity and relative stability in structure and hence are very likely present in serum/plasma. Meanwhile, since microRNAs are a new type of disease markers, it is anticipated that by studying whether or not microRNAs are present in serum/plasma, whether or not they can be detected and the connection between microRNAs and diseases, a new technology is established for the early disease diagnosis, disease identification as well as monitoring and controlling of course of diseases, prediction of malignant disease relapse and prognosis and complication occurrence, assessment of drug efficacy, guide of medication, individualized treatment, screening of active ingredients of Chinese Traditional Medicines, population taxonomy, etc., by use of the microRNAs stably existing in serum/plasma as well as their specificity changes.
The present invention provides a combination of microRNAs for evaluating physiological and/or pathological condition in a subject, wherein the combination comprises all detectable microRNAs stably existing in the serum/plasma of the subject.
The present invention further provides a method for evaluating physiological and/or pathological condition in a subject, wherein the method comprises determining all detectable microRNAs stably existing in the serum/plasma of the subject.
In the above-mentioned combination or method, all detectable microRNAs stably existing in serum/plasma of a subject may be all mature microRNAs in human serum/plasma, specifically include let-7a, let-7b, let-7c, let-7d, let-7e, let-7f, let-7g, let-7i, miR-1, miR-100, miR-101, miR-103, miR-105, miR-106a, miR-106b, miR-107, miR-10a, miR-10b, miR-122a, miR-124a, miR-125a, miR-125b, miR-126, miR-126*, miR-127, miR-128a, miR-128b, miR-129, miR-130a, miR-130b, miR-132, miR-133a, miR-133b, miR-134, miR-135a, miR-135b, miR-136, miR-137, miR-138, miR-139, miR-140, miR-141, miR-142-3p, miR-142-5p, miR-143, miR-144, miR-145, miR-146a, miR-146b, miR-147, miR-148a, miR-148b, miR-149, miR-150, miR-151, miR-152, miR-153, miR-154, miR-154*, miR-155, miR-15a, miR-15b, miR-16, miR-17-3p, miR-17-5p, miR-181a, miR-181b, miR-181c, miR-181d, miR-182, miR-182*, miR-183, miR-184, miR-185, miR-186, miR-187, miR-188, miR-189, miR-18a, miR-18a*, miR-18b, miR-190, miR-191, miR-191*, miR-192, miR-193a, miR-193b, miR-194, miR-195, miR-196a, miR-196b, miR-197, miR-198, miR-199a, miR-199a*, miR-199b, miR-19a, miR-19b, miR-200a, miR-200a*, miR-200b, miR-200c, miR-202, miR-202*, miR-203, miR-204, miR-205, miR-206, miR-208, miR-20a, miR-20b, miR-21, miR-210, miR-211, miR-212, miR-213, miR-214, miR-215 miR-216, miR-217, miR-218, miR-219, miR-22, miR-220, miR-221 miR-222, miR-223, miR-224, miR-23a, miR-23b, miR-24, miR-25, miR-26a, miR-26b, miR-27a, miR-27b, miR-28, miR-296, miR-299-3p, miR-299-5p, miR-29a, miR-29b, miR-29c, miR-301, miR-302a, miR-302a*, miR-302b, miR-302b*, miR-302c, miR-302c*, miR-302d, miR-30a-3p, miR-30a-5p, miR-30b, miR-30e, miR-30d, miR-30e-3p, miR-30e-5p, miR-32, miR-320, miR-323, miR-324-3p, miR-324-5p, miR-325, miR-326, miR-328, miR-329, miR-33, miR-330, miR-331, miR-335, miR-337, miR-338, miR-339, miR-33b, miR-340, miR-342, miR-345, miR-346, miR-34a, miR-34b, miR-34c, miR-361, miR-362, miR-363, miR-363*, miR-365, miR-367, miR-368, miR-369-3p, miR-369-5p, miR-370, miR-371, miR-372, miR-373, miR-373*, miR-374, miR-375, miR-376a, miR-376a*, miR-376b, miR-377, miR-378, miR-379, miR-380-3p, miR-380-5p, miR-381, miR-382, miR-383, miR-384, miR-409-3p, miR-409-5p, miR-410, miR-411, miR-412, miR-421, miR-422a, miR-422b, miR-423, miR-424, miR-425, miR-425-5p, miR-429, miR-431, miR-432, miR-432*, miR-433, miR-448, miR-449, miR-450, miR-451, miR-452, miR-452*, miR-453, miR-455, miR-483, miR-484, miR-485-3p, miR-485-5p, miR-486, miR-487a, miR-487b, miR-488, miR-489, miR-490, miR-491, miR-492, miR-493, miR-493-3p, miR-494, miR-495, miR-496, miR-497, miR-498, miR-499, miR-500, miR-501, miR-502, miR-503, miR-504, miR-505, miR-506, miR-507, miR-508, miR-509, miR-510, miR-511, miR-512-3p, miR-512-5p, miR-513, miR-514, miR-515-3p, miR-515-5p, miR-516-3p, miR-516-5p, miR-517*, miR-517a, miR-517b, miR-517c, miR-518a, miR-518a-2*, miR-518b, miR-518c, miR-518c*, miR-518d, miR-518e, miR-518f, miR-518f*, miR-519a, miR-519b, miR-519c, miR-519d, miR-519e, miR-519e*, miR-520a, miR-520a*, miR-520b, miR-520c, miR-520d, miR-520d*, miR-520e, miR-520f, miR-520g, miR-520h, miR-521, miR-522, miR-523, miR-524, miR-524*, miR-525, miR-525*, miR-526a, miR-526b, miR-526b*, miR-526c, miR-527, miR-532, miR-542-3p, miR-542-5p, miR-544, miR-545, miR-548a, miR-548b, miR-548c, miR-548d, miR-549, miR-550, miR-551a, miR-552, miR-553, miR-554, miR-555, miR-556, miR-557, miR-558, miR-559, miR-560, miR-561, miR-562, miR-563, miR-564, miR-565, miR-566, miR-567, miR-568, miR-569, miR-570, miR-571, miR-572, miR-573, miR-574, miR-575, miR-576, miR-577, miR-578, miR-579, miR-580, miR-581, miR-582, miR-583, miR-584, miR-585, miR-586, miR-587, miR-588, miR-589, miR-590, miR-591, miR-592, miR-593, miR-594, miR-595, miR-596, miR-597, miR-598, miR-599, miR-600, miR-601, miR-602, miR-603, miR-604, miR-605, miR-606, miR-607, miR-608, miR-609, miR-610, miR-611, miR-612, miR-613, miR-614, miR-615, miR-616, miR-617, miR-618, miR-619, miR-620, miR-621, miR-622, miR-623, miR-624, miR-625, miR-626, miR-627, miR-628, miR-629, miR-630, miR-631, miR-632, miR-633, miR-634, miR-635, miR-636, miR-637, miR-638, miR-639, miR-640, miR-641, miR-642, miR-643, miR-644, miR-645, miR-646, miR-647, miR-648, miR-649, miR-650, miR-651, miR-652, miR-653, miR-654, miR-655, miR-656, miR-657, miR-658, miR-659, miR-660, miR-661, miR-662, miR-663, miR-7, miR-9, miR-9*, miR-92, miR-93, miR-95, miR-96, miR-98, miR-99 and miR-99b.
The aforesaid method for determining all detectable microRNAs stably existing in serum/plasma of a subject is one or more selected from the group consisting of RT-PCR method, Real-time PCR method, Northern blotting method, RNase protection assay, Solexa sequencing technology and biochip method.
The aforesaid RT-PCR method includes the following steps:
(1) extracting the total RNA from the serum/plasma of a subject and obtaining cDNA samples by RNA reverse transcription reaction; or collecting serum/plasma samples from the subject and conducting reverse transcription reaction with serum/plasma being a buffer so as to prepare cDNA samples;
(2) designing a primer by use of microRNAs and conducting PCR reaction;
(3) conducting agarose gel electrophoresis of PCR products;
(4) observing agarose gel under ultraviolet lamp after EB staining.
The aforesaid real-time PCR method includes the following steps:
(1) extracting the total RNA from the serum/plasma of a subject and obtaining cDNA samples by RNA reverse transcription reaction; or collecting serum/plasma samples from the subject and conducting reverse transcription reaction with serum/plasma being a buffer so as to prepare cDNA samples;
(2) designing a primer by use of microRNAs;
(3) adding a fluorescent probe to conduct PCR reaction;
(4) detecting and comparing the variation in levels of microRNAs in the serum/plasma relative to those of microRNAs in normal serum/plasma.
The present invention further provides a kit for evaluating physiological and/or pathological condition of a subject, wherein the kit comprises the tools for determining all detectable microRNAs stably existing in the serum/plasma of the subject. The kit may comprises the primers of all mature microRNAs in human serum/plasma, specifically comprises the primers of let-7a, let-7b, let-7c, let-7d, let-7e, let-7f, let-7g, let-7i, miR-1, miR-100, miR-101, miR-103, miR-105, miR-106a, miR-106b, miR-107, miR-10a, miR-10b, miR-122a, miR-124a, miR-125a, miR-125b, miR-126, miR-126*, miR-127, miR-128a, miR-128b, miR-129, miR-130a, miR-130b, miR-132, miR-133a, miR-133b, miR-134, miR-135a, miR-135b, miR-136, miR-137, miR-138, miR-139, miR-140, miR-141, miR-142-3p, miR-142-5p, miR-143, miR-144, miR-145, miR-146a, miR-146b, miR-147, miR-148a, miR-148b, miR-149, miR-150, miR-151, miR-152, miR-153, miR-154, miR-154*, miR-155, miR-15a, miR-15b, miR-16, miR-17-3p, miR-17-5p, miR-181a, miR-181b, miR-181c, miR-181d, miR-182, miR-182*, miR-183, miR-184, miR-185, miR-186, miR-187, miR-188, miR-189, miR-18a, miR-18a*, miR-18b, miR-190, miR-191, miR-191*, miR-192, miR-193a, miR-193b, miR-194, miR-195, miR-196a, miR-196b, miR-197, miR-198, miR-199a, miR-199a*, miR-199b, miR-19a, miR-19b, miR-200a, miR-200a*, miR-200b, miR-200c, miR-202, miR-202*, miR-203, miR-204, miR-205, miR-206, miR-208, miR-20a, miR-20b, miR-21, miR-210, miR-211, miR-212, miR-213, miR-214, miR-215, miR-216, miR-217, miR-218, miR-219, miR-22, miR-220, miR-221, miR-222, miR-223, miR-224, miR-23a, miR-23b, miR-24, miR-25, miR-26a, miR-26b, miR-27a, miR-27b, miR-28, miR-296, miR-299-3p, miR-299-5p, miR-29a, miR-29b, miR-29c, miR-301, miR-302a, miR-302a*, miR-302b, miR-302b*, miR-302c, miR-302c*, miR-302d, miR-30a-3p, miR-30a-5p, miR-30b, miR-30c, miR-30d, miR-30e-3p, miR-30e-5p, miR-32, miR-320, miR-323, miR-324-3p, miR-324-5p, miR-325, miR-326, miR-328, miR-329, miR-33, miR-330, miR-331, miR-335, miR-337, miR-338, miR-339, miR-33b, miR-340, miR-342, miR-345, miR-346, miR-34a, miR-34b, miR-34c, miR-361, miR-362, miR-363, miR-363*, miR-365, miR-367, miR-368, miR-369-3p, miR-369-5p, miR-370, miR-371, miR-372, miR-373, miR-373*, miR-374, miR-375, miR-376a, miR-376a*, miR-376b, miR-377, miR-378, miR-379, miR-380-3p, miR-380-5p, miR-381, miR-382, miR-383, miR-384, miR-409-3p, miR-409-5p, miR-410, miR-411, miR-412, miR-421, miR-422a, miR-422b, miR-423, miR-424, miR-425, miR-425-5p, miR-429, miR-431, miR-432, miR-432*, miR-433, miR-448, miR-449, miR-450, miR-451, miR-452, miR-452*, miR-453, miR-455, miR-483, miR-484, miR-485-3p, miR-485-5p, miR-486, miR-487a, miR-487b, miR-488, miR-489, miR-490, miR-491, miR-492, miR-493, miR-493-3p, miR-494, miR-495, miR-496, miR-497, miR-498, miR-499, miR-500, miR-501, miR-502, miR-503, miR-504, miR-505, miR-506, miR-507, miR-508, miR-509, miR-510, miR-511, miR-512-3p, miR-512-5p, miR-513, miR-514, miR-515-3p, miR-515-5p, miR-516-3p, miR-516-5p, miR-517*, miR-517a, miR-517b, miR-517c, miR-518a, miR-518a-2*, miR-518b, miR-518c, miR-518c*, miR-518d, miR-518e, miR-518f, miR-518f*, miR-519a, miR-519b, miR-519c, miR-519d, miR-519e, miR-519e*, miR-520a, miR-520a*, miR-520b, miR-520c, miR-520d, miR-520d*, miR-520e, miR-520f, miR-520g, miR-520h, miR-521, miR-522, miR-523, miR-524, miR-524*, miR-525, miR-525*, miR-526a, miR-526b, miR-526b* miR-526c, miR-527, miR-532, miR-542-3p, miR-542-5p, miR-544, miR-545, miR-548a, miR-548b, miR-548c, miR-548d, miR-549, miR-550, miR-551a, miR-552, miR-553, miR-554, miR-555, miR-556, miR-557, miR-558, miR-559, miR-560, miR-561, miR-562, miR-563, miR-564, miR-565, miR-566, miR-567, miR-568, miR-569, miR-570, miR-571, miR-572, miR-573, miR-574, miR-575, miR-576, miR-577, miR-578, miR-579, miR-580, miR-581, miR-582, miR-583, miR-584, miR-585, miR-586, miR-587, miR-588, miR-589, miR-590, miR-591, miR-592, miR-593, miR-594, miR-595, miR-596, miR-597, miR-598, miR-599, miR-600, miR-601, miR-602, miR-603, miR-604, miR-605, miR-606, miR-607, miR-608, miR-609, miR-610, miR-611, miR-612, miR-613, miR-614, miR-615, miR-616, miR-617, miR-618, miR-619, miR-620, miR-621, miR-622, miR-623, miR-624, miR-625, miR-626, miR-627, miR-628, miR-629, miR-630, miR-631, miR-632, miR-633, miR-634, miR-635, miR-636, miR-637, miR-638, miR-639, miR-640, miR-641, miR-642, miR-643, miR-644, miR-645, miR-646, miR-647, miR-648, miR-649, miR-650, miR-651, miR-652, miR-653, miR-654, miR-655, miR-656, miR-657, miR-658, miR-659, miR-660, miR-661, miR-662, miR-663, miR-7, miR-9, miR-9*, miR-92, miR-93, miR-95, miR-96, miR-98, miR-99a and miR-99b.
The present invention also provides a biochip for evaluating physiological and/or pathological condition of a subject, wherein the biochip contains the components for determining all detectable microRNAs stably existing in the serum/plasma of the subject. The biochip may also contain the probes for all mature microRNAs in human serum/plasma. The probes specifically include the probes as shown in Table 1.
Specifically, among the above-mentioned combinations, methods, kits or biochips, the said evaluation of the physiological and/or pathological condition of a subject is to determine the physiological and/or pathological condition of the subject after being administrated a test sample, which is specifically useful for screening the test sample for the activities on the prevention and/or treatment of diseases; the said evaluation of the physiological and/or pathological condition of a subject is to diagnose and/or differentially diagnose the diseases of the subject; the said evaluation of the physiological and/or pathological condition of a subject is to evaluate the effectiveness of the treatment on the diseases of the subject; the said evaluation of the physiological and/or pathological condition of a subject is to predict the disease occurrence of the subject, which is specifically the occurrence of complications and/or the relapse of malignant diseases; the above-mentioned combinations, methods, kits or biochips can also be useful for detecting the subject for prohibited drugs-taking.
The above-mentioned diseases include a variety of tumors; various acute/chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute/chronic infectious diseases caused by various pathogenic microorganisms; other acute/chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular diseases, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary, diseases of reproductive system and diseases of locomotor system.
The above-mentioned serum/plasma derives from the living bodies, tissues, organs and/or corpuses of the subject.
The problems to be solved by the present invention include: (1) analyzing and identifying the microRNA molecules and their stability in serum/plasma of a variety of animals such as human, mice and rats; (2) studying the specificity changes of microRNAs in serum/plasma during the course of various clinical diseases including a variety of tumors; various acute/chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute/chronic infectious diseases caused by various pathogenic microorganisms; other acute/chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular diseases, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system; (3) detecting the respective changes of microRNAs in serum/plasma for different diseases through biochip and sequencing technology for microRNAs in serum/plasma; (4) screening a kind of microRNA molecules in serum/plasma which have relatively greater differential expression during the course of diseases and normal physiological conditions to develop detection technologies for serum/plasma microRNAs, and then preparing biochips and diagnostic kits useful for disease diagnosis etc.
Specifically, the present invention analyzes and identifies the existence of microRNA molecules in serum/plasma of various animals such as human, mice and rats through the methods of RT-PCR, Real-time PCR, Northern blotting, RNase protection assay, Solexa sequencing technology and biochip. The stability of microRNAs in serum/plasma is studied by comparing the changes of microRNAs by the effect of DNase and RNase. The existence of serum/plasma microRNAs molecules and the correctness of their sequences are further verified through sequencing and comparing the PCR products of serum/plasma microRNAs.
The detailed preparation and analysis for serum/plasma microRNAs are as follows:
RT-PCR method: collecting serum/plasma samples; conducting reverse transcription reaction on serum/plasma samples to prepare cDNA samples, or extracting total RNA of serum/plasma with Trizol reagent and then conducting reverse transcription reaction so as to prepare cDNA samples; designing a primer through mature microRNAs so as to conduct PCR reaction; carrying out agarose gel electrophoresis with the products of PCR; and observing and taking photographs for the results under ultraviolet lamp after EB staining.
Real-time PCR method: collecting serum/plasma samples; conducting reverse transcription reaction on serum/plasma samples to prepare cDNA samples, or extracting total RNA of serum/plasma with Trizol reagent and then conducting reverse transcription reaction so as to prepare cDNA samples; designing a primer of PCR through mature microRNAs and adding a fluorescent probe EVA GREEN so as to carry out PCR reaction; analyzing and processing the data and then comparing the results.
Northern blotting method: collecting serum/plasma samples; extracting total RNA of serum/plasma with Trizol reagent; conducting denaturing PAGE-electrophoresis and membrane transferring experiment; preparing isotope-labeled microRNA probes; conducting membrane hybridization reaction; detecting the isotope signal for results such as using phosphor-screen scanning technology.
RNase protection assay: firstly synthesizing an antisense RNA probe, labelling it with isotopes and purifying it; collecting serum/plasma samples and extracting RNA; dissolving the extracted DNA in a hybrid buffer and then adding an antisense RNA probe so as to conduct hybridization reaction; adding a RNase digestion solution to initate reaction; subjecting the resultant material to electrophoresis and radioautography; and analyzing the results.
Solexa sequencing technology: collecting serum/plasma samples; extracting total RNA of serum/plasma with Trizol reagent; conducting PAGE-electrophoresis to recover RNA molecules of 17˜27 nt; enzyme-linking adaptor prime to the 3′ and 5′ end of small RNA molecules respectively; conducting RT-PCR reaction prior to sequencing; and analyzing and processing the data.
Biochip method: arraying a library of all over 500 mature microRNAs to prepare biochips; collecting serum/plasma samples; extracting total RNA of serum/plasma; separating microRNAs by column separation; fluorescently-labelling microRNAs by use of T4 RNA ligase; conducting hybridization reaction with a biochip; and detecting and analyzing the data.
The change trend and change volume of serum/plasma microRNAs during various diseases and their relevancy with various diseases are analyzed through the above-mentioned technologies of RT-PCR, Real-time PCR, Northern blotting, RNase protection assay, Solexa sequencing technology, Biochip, etc. Among others, what to do firstly is to detect and analyze the changes of let-7a, let-7b, let-7c, let-7d, let-7e, let-7f, let-7g, let-7i, miR-1, miR-100, miR-101, miR-103, miR-105, miR-106a, miR-106b, miR-107, miR-10a, miR-10b, miR-122a, miR-124a, miR-125a, miR-125b, miR-126, miR-126*, miR-127, miR-128a, miR-128b, miR-129, miR-130a, miR-130b, miR-132, miR-133a, miR-133b, miR-134, miR-135a, miR-135b, miR-136, miR-137, miR-138, miR-139, miR-140, miR-141, miR-142-3p, miR-142-5p, miR-143, miR-144, miR-145, miR-146a, miR-146b, miR-147, miR-148a, miR-148b, miR-149, miR-150, miR-151, miR-152, miR-153, miR-154, miR-154*, miR-155, miR-15a, miR-15b, miR-16, miR-17-3p, miR-17-5p, miR-181a, miR-181b, miR-181c, miR-181d, miR-182, miR-182*, miR-183, miR-184, miR-185, miR-186, miR-187, miR-188, miR-189, miR-18a, miR-18a*, miR-18b, miR-190, miR-191, miR-191*, miR-192, miR-193a, miR-193b, miR-194, miR-195, miR-196a, miR-196b, miR-197, miR-198, miR-199a, miR-199a*, miR-199b, miR-19a, miR-19b, miR-200a, miR-200a*, miR-200b, miR-200c, miR-202, miR-202*, miR-203, miR-204, miR-205, miR-206, miR-208, miR-20a, miR-20b, miR-21, miR-210, miR-211, miR-212, miR-213, miR-214, miR-215, miR-216, miR-217, miR-218, miR-219, miR-22, miR-220, miR-221, miR-222, miR-223, miR-224, miR-23a, miR-23b, miR-24, miR-25, miR-26a, miR-26b, miR-27a, miR-27b, miR-28, miR-296, miR-299-3p, miR-299-5p, miR-29a, miR-29b, miR-29c, miR-301, miR-302a, miR-302a*, miR-302b, miR-302b*, miR-302c, miR-302c*, miR-302d, miR-30a-3p, miR-30a-5p, miR-30b, miR-30c, miR-30d, miR-30e-3p, miR-30e-5p, miR-31, miR-32, miR-320, miR-323, miR-324-3p, miR-324-5p, miR-325, miR-326, miR-328, miR-329, miR-33, miR-330, miR-331, miR-335, miR-337, miR-338, miR-339, miR-33b, miR-340, miR-342, miR-345, miR-346, miR-34a, miR-34b, miR-34c, miR-361, miR-362, miR-363, miR-363*, miR-365, miR-367, miR-368, miR-369-3p, miR-369-5p, miR-370, miR-371, miR-372, miR-373, miR-373*, miR-374, miR-375, miR-376a, miR-376a*, miR-376b, miR-377, miR-378, miR-379, miR-380-3p, miR-380-5p, miR-381, miR-382, miR-383, miR-384, miR-409-3p, miR-409-5p, miR-410, miR-411, miR-412, miR-421, miR-422a, miR-422b, miR-423, miR-424, miR-425, miR-425-5p, miR-429, miR-431, miR-432 miR-432*, miR-433, miR-448, miR-449, miR-450, miR-451, miR-452, miR-452*, miR-453, miR-455, miR-483, miR-484, miR-485-3p, miR-485-5p, miR-486, miR-487a, miR-487b, miR-488, miR-489, miR-490, miR-491, miR-492, miR-493, miR-493-3p, miR-494, miR-495, miR-496, miR-497, miR-498, miR-499, miR-500, miR-501, miR-502, miR-503, miR-504, miR-505, miR-506, miR-507, miR-508, miR-509, miR-510, miR-511, miR-512-3p, miR-512-5p, miR-513, miR-514, miR-515-3p, miR-515-5p, miR-516-3p, miR-516-5p, miR-517*, miR-517a, miR-517b, miR-517c, miR-518a, miR-518a-2*, miR-518b, miR-518c, miR-518c*, miR-518d, miR-518e, miR-518f, miR-518f*, miR-519a, miR-519b, miR-519c, miR-519d, miR-519e, miR-519e*, miR-520a, miR-520a*, miR-520b, miR-520c miR-520d, miR-520d*, miR-520e, miR-520f, miR-520g, miR-520h, miR-521, miR-522, miR-523, miR-524, miR-524*, miR-525, miR-525*, miR-526a, miR-526b, miR-526b*, miR-526c, miR-527, miR-532, miR-542-3p, miR-542-5p, miR-544, miR-545, miR-548a, miR-548b, miR-548c, miR-548d, miR-549, miR-550, miR-551a, miR-552, miR-553, miR-554, miR-555, miR-556, miR-557, miR-558, miR-559, miR-560, miR-561, miR-562, miR-563, miR-564, miR-565, miR-566, miR-567, miR-568, miR-569, miR-570, miR-571, miR-572, miR-573, miR-574, miR-575, miR-576, miR-577, miR-578, miR-579, miR-580, miR-581, miR-582, miR-583, miR-584, miR-585, miR-586, miR-587, miR-588, miR-589, miR-590, miR-591, miR-592, miR-593, miR-594, miR-595, miR-596, miR-597, miR-598, miR-599, miR-600, miR-601, miR-602, miR-603, miR-604, miR-605, miR-606, miR-607, miR-608, miR-609, miR-610, miR-611 miR-612, miR-613, miR-614, miR-615, miR-616, miR-617, miR-618, miR-619, miR-620, miR-621, miR-622, miR-623, miR-624, miR-625, miR-626, miR-627, miR-628, miR-629, miR-630, miR-631, miR-632, miR-633, miR-634, miR-635, miR-636, miR-637, miR-638, miR-639, miR-640, miR-641, miR-642, miR-643, miR-644, miR-645, miR-646, miR-647, miR-648, miR-649, miR-650, miR-651, miR-652, miR-653, miR-654, miR-655, miR-656, miR-657, miR-658, miR-659, miR-660, miR-661, miR-662, miR-663, miR-7, miR-9, miR-9*, miR-92, miR-93, miR-95, miR-98, miR-99a and miR-99b in various clinical diseases (including a variety of tumors; various acute/chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute/chronic infectious diseases caused by various pathogenic microorganisms; other acute/chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular diseases, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system); Biochips of serum/plasma microRNAs are prepared to determine the changes of serum/plasma microRNAs in different diseases, and meanwhile, Solexa sequencing and analysis on microRNAs in serum/plasma in different diseases are conducted.
The research and development of a technology for detecting disease-related serum/plasma microRNAs. Specifically, the microRNAs with disease-related specificity changes are screened out, their primers are collected into a PCR kit (RT-PCR or Real-time PCR) to prepare a disease-diagnostic kit, or their reverse complementary sequences are dripped on chips as probes so as to prepare the biochips for detecting serum/plasma microRNAs specific for a certain disease.
Presently, the technologies of traditional biochemistry and molecular biology for the clinical diagnosis of diseases are relatively complicated and insensitive. Novel techniques developed in recent years possibly useful for disease diagnosis are gene chip technique, protein (antibody) chip technique, etc. The changes at mRNA level measured through gene chips cannot completely reflect the actual changes at protein level, since the bioactivity of protein is closely related to post-transcriptional modification such as glycosylation and phosphorylation. In addition, for detection of many diseases, marker molecules in body fluids and blood cannot be detected through gene chip technology. Meanwhile, protein (antibody) chip technique and proteomic techniques also bear their limitations. In human body, especially in serum/plasma, there are tens of thousands of protein and polypeptide segments with extensively distributed concentrations, and the number of proteins definitely reported is very small, let alone those quantified. It is an extremely arduous task to find out those proteins having close relation with specific diseases from the large quantity of proteins and understand their roles in histopathologic changes. Moreover, lacking of complete antibody resources is the bottleneck restraining the development of antibody biochip technology. The detection technology for serum/plasma microRNAs based on biochips of serum/plasma microRNAs and diagnostic kits skillfully combines the peculiar properties of serum/plasma microRNAs with conventional molecular biology detection technique together, which can rapidly analyze the respective constitution of serum/plasma microRNAs in respect of various diseases with high throughput and hence be of extremely clinical practicality. Since the changes of physiological conditions in organs and tissues will cause the constitutional changes of serum/plasma microRNAs, serum/plasma microRNAs can be used as “fingerprints for diseases” to realize early diagnosis of diseases.
The advantages of the technology of detecting serum/plasma microRNAs are as follows:
(1) As novel disease markers, serum/plasma microRNAs possess certain advantages such as extensive spectrum for detection, high sensitivity, low cost for detection, convenient sampling, easy preservation for samples (preserving serum/plasma at −20° C. will do), etc. This method can be widely used in general survey of diseases and other relevant tasks and has become an efficient means for early diagnosis of diseases.
(2) As novel disease markers, serum/plasma microRNAs will improve the low-specificity and low-sensitivity caused by individual differences which single markers are difficult to overcome, and notably increase the clinical detection rate of diseases so as to realize early diagnosis of diseases.
(3) The advantages of the technology of detecting serum/plasma microRNAs lie in that what to be detected is series of disease related markers, thus it can address the differences (i.e., age, sex, race, diet, circumstance, etc.) between individual patients, which are exactly a primary problem difficult to overcome by single disease markers.
In summary, utilizing the technology of detecting serum/plasma microRNAs can confirm diagnosis of histopathologic changes in early stage. These novel serum/plasma markers not only provide material foundation for people to comprehensively understand the mechanism of histopathologic changes in molecule level, but also accelerate the progress in diagnostics and therapeutics of clinical diseases. Of course, a majority of molecular diagnostic techniques used for disease detection in early period are at initial experimental stage and their validity needs to be further verified and improved. Moreover, since every disease has the characteristics of its own, this requires a peculiar method for the detection of said disease. In this manner, it is impossible for all diseases to be detected out only through one or only a few of detection methods. Nevertheless, based on the superiority of serum/plasma microRNAs, it is believed that, in the near future, the diagnostic technique of serum/plasma microRNAs for severe diseases such as cancer will become part of routine physical examination. In addition, microRNA related gene therapy will be widely utilized. Consequently, the overcoming of these diseases will come true, not just a dream.
The following are the detailed description of the embodiments of this invention with reference to the drawings, wherein:
In
The RT-PCR Experiments of MicroRNAs in Serum/Plasma
By using RT-PCR technique, it is found and proved that there stably exist various microRNAs in serum/plasma of both human beings and animals, and that their expression levels are considerably high. The specific RT-PCR steps are as follows:
(1) collecting serum/plasma of mice, rats, normal persons and some patients;
(2) preparing samples of cDNA. This operation has two options: one is to directly conduct reverse transcription reaction using 10 μl of serum/plasma; the other is to firstly extract the total RNA from serum/plasma (usually, about 10 μg of RNA can be enriched from 10 ml of serum/plasma) with Trizol reagent (Invitrogen Co.), subsequently obtain cDNA through RNA reverse transcription reaction. The reaction system of reverse transcription includes 4 μl 5×AMV buffer, 2 μl 10 mM each dNTP mixture (Takara Co.), 0.5 μl RNase Inhibitor (Takara Co.), 2 μl AMY (Takara Co.) and 1.5 μl gene specific reverse primers mixtures. The reaction steps successively include 15 minutes of incubation at 16° C., 1 hour of reaction at 42° C. and 5 minutes of incubation at 85° C.;
(3) PCR and Electrophoresis observation. The cDNA is diluted by 1/50. To 1 μl diluted cDNA are added 0.3 μl Taq polymerase (Takara Co.), 0.2 μl 10 μM forward primer, 0.20 μl 10 μM universal reverse primer, 1.2 μl 25 mM MgCl2, 1.6 μl 2.5 mM each dNTP mixture (Takara Co.), 2 μl 10×PCR buffer, 13.5 μl H2O, and PCR reaction is conducted in the 20 μl system. The PCR reaction is done under the following conditions: one cycle at 95° C. for 5 mins followed by 40 cycles at 95° C. for 15 seconds and 60° C. for 1 minute. 10 μl PCR product is subjected to 3% Agarose Gel Electrophoresis, which is observed under ultraviolet lamp after EB staining.
The detailed experimental results are shown in
To further verify that there stably exist the microRNAs in serum/plasma, RNA is firstly extracted from the serum of normal persons, then all over 500 mature microRNAs of human are selected for PCR experiment. As shown in
Quantitative PCR experiments of microRNAs in serum/plasma are conducted to study the specific variation of microRNAs quantity in serum/plasma during the course of various diseases, including various tumors, various acute and chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute and chronic infectious diseases caused by various pathogenic microorganisms; other acute and chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular disease, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system. The experimental principles and experimental steps of quantitative PCR are basically the same as those of RT-PCR, with the only difference between them being the addition of a fluorescent dye EVA GREEN in the process of PCR. An ABI Prism 7300 fluorescent quantitative PCR instrument is used to conduct PCR reaction under the following conditions: one cycle at 95° C. for 5 mins followed by 40 cycles at 95° C. for 15 seconds and 60° C. for 1 minute. The data processing method used is ΔΔCT method, wherein CT is the number of cycles when the reaction reaches the threshold. The expression level of each microRNAs relative to that of internal standard reference can be expressed by the equation of 2-ACT, wherein ΔCT=CTsample−CTinternal reference. Reverse transcription reactions are directly conducted on serum/plasma samples of a patient and those of a normal person, and the quantities of microRNAs contained in each sample of serum/plasma are compared through quantitative PCR reactions.
Serum samples of patients who suffer from aplastic anemia, breast cancer, osteosarcoma, CNS (Central Nervous System) lymphoma, diabetes are selected, and at the same time, all over 500 mature microRNAs of human beings are used to conduct PCR reaction experiments.
Through detecting the quantities of microRNAs and macroRNAs in serum and blood cells, it is found that there is an abundant content of microRNAs in serum. See
It is also found that microRNAs are to some extent able to resist the action of endonuclease, which is possibly one of the reasons why microRNAs can stably exist in serum/plasma. Total RNAs extracted from cultured cell line are processed with endonuclease RNase A and the remaining quantity of macroRNAs and microRNAs are then detected. As shown in
Based on the two characteristics of abundance in content and stable existence of microRNAs in serum/plasma, microRNAs could be well applied in clinical test.
Example 4 Preparation of the Biochip of Serum/Plasma MicroRNAs Useful for Disease DiagnosisA biochip of serum/plasma microRNAs is fabricated to verify the reliability of a kind of serum/plasma microRNAs probes relating to diseases which are selected through quantitative PCR method. The biochip contains all microRNAs probes that can be normally detected in people's serum/plasma, constituting a probe library. See Table 1.
When the probes are specifically applied in certain disease diagnosis or efficacy screening, some probes of the probe library are put together to construct a probe collection which makes it possible to quantitatively detect the variation of microRNAs in the specific conditions. For example, when diagnosing colon cancer, the collection of probes that have interaction with microRNAs of numbers 17-5p, 21, 103, 106a, 107, 126*, 143, 145, 150, 155 and 210 is used. For another example, when diagnosing myocardial hypertrophy and chronic heart failure, the collection of probes that have interaction with microRNAs of numbers 21, 23a, 23b, 24, 27a, 27b, 125b, 195, 199a, 214, 217, 133a is used. In addition, the chip can also do high-throughput screening of the probes of microRNAs varying stably in serum/plasma, and diseases can be predicted and diagnosed based on the overall variation of microRNAs in serum/plasma.
Sequencing method or quantitative PCR method is firstly used to determine that there is more than one copy of microRNAs in serum/plasma, and then reverse complementary probes of these microRNAs are synthesized, after which these probes are spotted on a chemically-modified slide in a size of 75×25 mm using a biochip microarrayer SmartArray™. The samples spotted on the chip also include U6 and tRNA as internal standard, artificially-prepared external standard in length of 30 bases, Hex as positive control etc. The entire lattice is divided into 4 sub-lattices and each sub-lattice has 23 rows and 21 columns, wherein the spot distance is 185 mm and the spot diameter is about 130 μm and each probe was repeatly spotted for 3 times.
The operational procedure of the biochip is: (1) extracting the total RNA from serum/plasma and detecting its quality through formaldehyde denaturing gel electrophoresis; (2) separation of microRNAs: 50-100 μg total RNA is taken to separate microRNAs from total RNA with Ambion's miRNA Isolation Kit (Cat #. 1560); (3) fluorescently-labeling of microRNAs samples: microRNAs samples are fluorescently-labeling with T4 RNA ligase, then precipitated with absolute ethanol, and then blown to dryness for chip hybridization; (4) hybridization and cleaning: RNA is dissolved into 16 μL hybridizing solution (15% formamide, 0.2% SDS, 3×SSC and 50×Denhardt's solution), and hybridized at 420 overnight. After completion of the hybridization, it is washed in a solution containing 0.2% SDS and 2×SSC at about 42° C. for 4 minutes, and then washed in a solution containing 0.2×SSC at room temperature for 4 minutes. Thereafter, the slides can be used for scanning immediately after being dried; (5) chip scanning: the chip is scanned with two-channel laser scanner LuxScan 10K/A; (6) data extracting and analysis: the chip image is analyzed with an image analyzing software LuxScan 3.0, the image signal is transformed into digital signal, and finally differentially-expressed genes are analyzed and selected with SAM method.
A biochip is prepared as above by using a kind of serum/plasma microRNAs probes which express greatly differently under disease condition and normal physiological condition double-verified by quantitative PCR technique and biochip technique. As compared with the traditional chip, there is no significant improvement in the manufacturing process and operational procedure of this biochip, but this chip simplifies the probe library, thereby greatly reducing the manufacturing cost and production time of the chip, and hence is easy to prepare. Meanwhile it increases the pertinence and practicability of chip. The application of the chip in practice can detect diseases in an early phase with only need of the serum/plasma of a patient and no need of other tissues, which helps guide the diagnosis and treatment.
Example 5 Preparation of Kits of MicroRNAs Useful for Disease Diagnosis and PredictionThe manufacturing processed and operational procedures of microRNAs kits useful for diagnosis, prediction of complication occurrence and malignant disease relapse, evaluation of therapeutic effects, screening of pharmaceutical active ingredients, assessment of drug efficacy, forensic authentication and prohibited drug inspection, etc. of all diseases are based on quantitative PCR technique and semi-quantitative PCR technique and biochip technique. The above-mentioned diseases include various tumors; various acute/chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute/chronic infectious diseases caused by various pathogenic microorganisms; other acute/chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular diseases, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system.
Sequencing method or quantitative PCR method is firstly used to determine that there is more than one copy of microRNAs in serum/plasma. Then, a kind of serum/plasma microRNAs that have a big difference between the expression levels in disease condition and in normal physiological condition are screened out through the techniques of quantative PCR and biochip, which are taken as an indicator for predicting whether canceration or other disease occurs and diagnosing the pathological degree. Finally the number of screened corresponding serum/plasma microRNAs of each disease would be controlled to over ten to tens, which is the optimized condensement of the chip-probe library. The kit contains a batch of serum/plasma microRNAs primers, Taq polymerase, dNTP, etc. The value of the kit lies in making it possible to detect the changing trend of microRNAs through the most simplified probe library and with only need of serum/plasma and no need of any other tissue samples, and further predict the probability of occurrence of diseases or diagnose the pathological phase of diseases based on this changing trend detected. Thus, the application of this kit in practice can increase the possibility of discovering diseases in an early phase, which helps guide the diagnosis and treatment of diseases.
Claims
1. A combination of microRNAs for evaluating the physiological and/or pathological condition of a subject, wherein the combination comprises all detectable microRNAs stably existing in the serum/plasma of the subject.
2. The combination according to claim 1, characterized in that said all detectable microRNAs stably existing in the serum/plasma of a subject are all mature microRNAs in human serum/plasma.
3. The combination according to claim 1, characterized in that said all detectable microRNAs stably existing in the serum/plasma of a subject are let-7a, let-7b, let-7c, let-7d, let-7e, let-7f, let-7g, let-7i, miR-1, miR-100, miR-101, miR-103, miR-105, miR-106a, miR-106b, miR-107, miR-10a, miR-10b, miR-122a, miR-124a, miR-125a, miR-125b, miR-126, miR-126*, miR-127, miR-128a, miR-128b, miR-129, miR-130a, miR-130b, miR-132, miR-133a, miR-133b, miR-134, miR-135a, miR-135b, miR-136, miR-137, miR-138, miR-139, miR-140, miR-141, miR-142-3p, miR-142-5p, miR-143, miR-144, miR-145, miR-146a, miR-146b, miR-147, miR-148a, miR-148b, miR-149, miR-150, miR-151, miR-152, miR-153, miR-154, miR-154*, miR-155, miR-15a, miR-15b, miR-16, miR-17-3p, miR-17-5p, miR-181a, miR-181b, miR-181c, miR-181d, miR-182, miR-182*, miR-183, miR-184, miR-185, miR-186, miR-187, miR-188, miR-189, miR-18a, miR-18a*, miR-18b, miR-190, miR-191, miR-191*, miR-192, miR-193a, miR-193b, miR-194, miR-195, miR-196a, miR-196b, miR-197, miR-198, miR-199a, miR-199a*, miR-199b, miR-19a, miR-19b, miR-200a, miR-200a*, miR-200b, miR-200c, miR-202, miR-202*, miR-203, miR-204, miR-205, miR-206, miR-208, miR-20a, miR-20b, miR-21, miR-210, miR-211, miR-212, miR-213, miR-214, miR-215, miR-216, miR-217, miR-218, miR-219, miR-22, miR-220, miR-221, miR-222, miR-223, miR-224, miR-23a, miR-23b, miR-24, miR-25, miR-26a, miR-26b, miR-27a, miR-27b, miR-28, miR-296, miR-299-3p, miR-299-5p, miR-29a, miR-29b, miR-29c, miR-301, miR-302a, miR-302a*, miR-302b, miR-302b*, miR-302c, miR-302c*, miR-302d, miR-30a-3p, miR-30a-5p, miR-30b, miR-30c, miR-30d, miR-30e-3p, miR-30e-5p, miR-31, miR-32, miR-320, miR-323, miR-324-3p, miR-324-5p, miR-325, miR-326, miR-328, miR-329, miR-33, miR-330, miR-331, miR-335, miR-337, miR-338, miR-339, miR-33b, miR-340, miR-342, miR-345, miR-346, miR-34a, miR-34b, miR-34c, miR-361, miR-362, miR-363, miR-363*, miR-365, miR-367, miR-368, miR-369-3p, miR-369-5p, miR-370, miR-371, miR-372, miR-373, miR-373*, miR-374, miR-375, miR-376a, miR-376a*, miR-376b, miR-377, miR-378, miR-379, miR-380-3p, miR-380-5p, miR-381, miR-382, miR-383, miR-384, miR-409-3p, miR-409-5p, miR-410, miR-411, miR-412, miR-421, miR-422a, miR-422b, miR-423, miR-424, miR-425, miR-425-5p, miR-429, miR-431, miR-432, miR-432*, miR-433, miR-448, miR-449, miR-450, miR-451, miR-452, miR-452*, miR-453, miR-455, miR-483, miR-484, miR-485-3p, miR-485-5p, miR-486, miR-487a, miR-487b, miR-488, miR-489, miR-490, miR-491, miR-492, miR-493, miR-493-3p, miR-494, miR-495, miR-496, miR-497, miR-498, miR-499, miR-500, miR-501, miR-502, miR-503, miR-504, miR-505, miR-506, miR-507, miR-508, miR-509, miR-510, miR-511, miR-512-3p, miR-512-5p, miR-513, miR-514, miR-515-3p, miR-515-5p, miR-516-3p, miR-516-5p, miR-517*, miR-517a, miR-517b, miR-517c, miR-518a, miR-518a-2*, miR-518b, miR-518c, miR-518c*, miR-518d, miR-518e, miR-518f, miR-518f*, miR-519a, miR-519b, miR-519c, miR-519d, miR-519e, miR-519e*, miR-520a, miR-520a*, miR-520b, miR-520c, miR-520d, miR-520d*, miR-520e, miR-520f, miR-520g, miR-520h, miR-521, miR-522, miR-523, miR-524, miR-524*, miR-525, miR-525*, miR-526a, miR-526b, miR-526b*, miR-526c, miR-527, miR-532, miR-542-3p, miR-542-5p, miR-544, miR-545, miR-548a, miR-548b, miR-548c, miR-548d, miR-549, miR-550, miR-551a, miR-552, miR-553, miR-554, miR-555, miR-556, miR-557, miR-558, miR-559, miR-560, miR-561, miR-562, miR-563, miR-564, miR-565, miR-566, miR-567, miR-568, miR-569, miR-570, miR-571, miR-572, miR-573, miR-574, miR-575, miR-576, miR-577, miR-578, miR-579, miR-580, miR-581, miR-582, miR-583, miR-584, miR-585, miR-586, miR-587, miR-588, miR-589, miR-590, miR-591, miR-592, miR-593, miR-594, miR-595, miR-596, miR-597, miR-598, miR-599, miR-600, miR-601, miR-602, miR-603, miR-604, miR-605, miR-606, miR-607, miR-608, miR-609, miR-610, miR-611, miR-612, miR-613, miR-615, miR-616, miR-617, miR-618, miR-619, miR-620, miR-621, miR-622, miR-623, miR-624, miR-625, miR-626, miR-627, miR-628, miR-629, miR-630, miR-631, miR-632, miR-633, miR-634, miR-635, miR-636, miR-637, miR-638, miR-639, miR-640, miR-641, miR-642, miR-643, miR-644, miR-645, miR-646, miR-647, miR-648, miR-649, miR-650, miR-651, miR-652, miR-653, miR-654, miR-655, miR-656, miR-657, miR-658, miR-659, miR-660, miR-661, miR-662, miR-663, miR-7, miR-9, miR-9*, miR-92, miR-93, miR-95, miR-96, miR-98, miR-99a and miR-99b.
4. The combination according to claim 1, characterized in that said evaluating the physiological and/or pathological condition of a subject is to determine physiological and/or pathological condition of the subject after being administrated a test sample.
5. The combination according to claim 4, characterized in that the combination is useful for screening the test sample for the activities on the prevention and/or treatment of diseases.
6. The combination according claim 1, characterized in that said evaluating the physiological and/or pathological condition of a subject is to diagnose and/or differentially diagnose the diseases of the subject.
7. The combination according to claim 1, characterized in that said evaluating the physiological and/or pathological condition of a subject is to evaluate the effectiveness of treating the diseases of the subject.
8. The combination of according to claim 1, characterized in that said evaluating the physiological and/or pathological condition of a subject is to predict the occurrence of diseases of the subject.
9. The combination according to claim 8, characterized in that the occurrence of diseases is the occurrence of complications and/or the relapse of malignant diseases.
10. The combination according to claim 5, characterized in that the diseases include various tumors; various acute and chronic infectious diseases, e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute and chronic infectious diseases caused by various pathogenic microorganisms; other acute and chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular diseases, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system.
11. The combination according to claim 1, characterized in that the combination is useful for detecting the subject for prohibited drugs-taking.
12. The combination according to claim 1, characterized in that the serum/plasma derives from living body, tissues, organs and/or corpuses of the subject.
13. A method for evaluating the physiological and/or pathological condition of a subject, wherein the method comprises determining all detectable microRNAs stably existing in serum/plasma of the subject.
14. The method according to claim 13, characterized in that said all detectable microRNAs stably existing in serum/plasma of a subject are all mature microRNAs in human serum/plasma.
15. The method according to claim 13, characterized in that said all detectable microRNAs stably existing in serum/plasma of a subjects are let-7a, let-7b, let-7c, let-7d, let-7e, let-7f, let-7g, let-7i, miR-1, miR-100, miR-101, miR-103, miR-105, miR-106a, miR-106b, miR-107, miR-10a, miR-10b, miR-122a, miR-124a, miR-125a, miR-125b, miR-126, miR-126*, miR-127, miR-128a, miR-128b, miR-129, miR-130a, miR-130b, miR-132, miR-133a, miR-133b, miR-134, miR-135a, miR-135b, miR-136, miR-137, miR-138, miR-139, miR-140, miR-141, miR-142-3p, miR-142-5p, miR-143, miR-144, miR-145, miR-146a, miR-146b, miR-147, miR-148a, miR-148b, miR-149, miR-150, miR-151, miR-152, miR-153, miR-154, miR-154*, miR-155, miR-15a, miR-15b, miR-16, miR-17-3p, miR-17-5p, miR-181a, miR-181b, miR-181c, miR-181d, miR-182, miR-182*, miR-183, miR-184, miR-185, miR-186, miR-187, miR-188, miR-189, miR-18a, miR-18a*, miR-18b, miR-190, miR-191, miR-191*, miR-192, miR-193a, miR-193b, miR-194, miR-195, miR-196a, miR-196b, miR-197, miR-198, miR-199a, miR-199a*, miR-199b, miR-19a, miR-19b, miR-200a, miR-200a*, miR-200b, miR-200c, miR-202, miR-202*, miR-203, miR-204, miR-205, miR-206, miR-208, miR-20a, miR-20b, miR-21, miR-210, miR-211, miR-212, miR-213, miR-214, miR-215, miR-216, miR-217, miR-218, miR-219, miR-22, miR-220, miR-221, miR-222, miR-223, miR-224, miR-23a, miR-23b, miR-24, miR-25, miR-26a, miR-26b, miR-27a, miR-27b, miR-28, miR-296, miR-299-3p, miR-299-5p, miR-29a, miR-29b, miR-29c, miR-301, miR-302a, miR-302a*, miR-302b, miR-302b*, miR-302c, miR-302c*, miR-302d, miR-30a-3p, miR-30a-5p, miR-30b, miR-30c, miR-30d, miR-30e-3p, miR-30e-5p, miR-31, miR-32, miR-320, miR-323, miR-324-3p, miR-324-5p, miR-325, miR-326, miR-328, miR-329, miR-33, miR-330, miR-331, miR-335, miR-337, miR-338, miR-339, miR-33b, miR-340, miR-342, miR-345, miR-346, miR-34a, miR-34b, miR-34c, miR-361, miR-362, miR-363, miR-363*, miR-365, miR-367, miR-368, miR-369-3p, miR-369-5p, miR-370, miR-371, miR-372, miR-373, miR-373*, miR-374, miR-375, miR-376a, miR-376a*, miR-376b, miR-377, miR-378, miR-379, miR-380-3p, miR-380-5p, miR-381, miR-382, miR-383, miR-384, miR-409-3p, miR-409-5p, miR-410, miR-411, miR-412, miR-421, miR-422a, miR-422b, miR-423, miR-424, miR-425, miR-425-5p, miR-429, miR-431, miR-432, miR-432*, miR-433, miR-448, miR-449, miR-450, miR-451, miR-452, miR-452*, miR-453, miR-455, miR-483, miR-484, miR-485-3p, miR-485-5p, miR-486, miR-487a, miR-487b, miR-488, miR-489, miR-490, miR-491, miR-492, miR-493, miR-493-3p, miR-494, miR-495, miR-496, miR-497, miR-498, miR-499, miR-500, miR-501, miR-502, miR-503, miR-504, miR-505, miR-506, miR-507, miR-508, miR-509, miR-510, miR-511, miR-512-3p, miR-512-5p, miR-513, miR-514, miR-515-3p, miR-515-5p, miR-516-3p, miR-516-5p, miR-517*, miR-517a, miR-517b, miR-517c, miR-518a, miR-518a-2*, miR-518b, miR-518c, miR-518c*, miR-518d, miR-518e, miR-518f, miR-518f*, miR-519a, miR-519b, miR-519c, miR-519d, miR-519e, miR-519e*, miR-520a, miR-520a*, miR-520b, miR-520c, miR-520d, miR-520d*, miR-520e, miR-520f, miR-520g, miR-520h, miR-521, miR-522, miR-523, miR-524, miR-524*, miR-525, miR-525*, miR-526a, miR-526b, miR-526b*, miR-526c, miR-527, miR-532, miR-542-3p, miR-542-5p, miR-544, miR-545, miR-548a, miR-548b, miR-548c, miR-548d, miR-549, miR-550, miR-551a, miR-552, miR-553, miR-554, miR-555, miR-556, miR-557, miR-558, miR-559, miR-560, miR-561, miR-562, miR-563, miR-564, miR-565, miR-566, miR-567, miR-568, miR-569, miR-570, miR-571, miR-572, miR-573, miR-574, miR-575, miR-576, miR-577, miR-578, miR-579, miR-580, miR-581, miR-582, miR-583, miR-584, miR-585, miR-586, miR-587, miR-588, miR-589, miR-590, miR-591, miR-592, miR-593, miR-594, miR-595, miR-596, miR-597, miR-598, miR-599, miR-600, miR-601, miR-602, miR-603, miR-604, miR-605, miR-606, miR-607, miR-608, miR-609, miR-610, miR-611, miR-612, miR-613, miR-614, miR-615, miR-616, miR-617, miR-618, miR-619, ma-620, miR-621, miR-622, miR-623, miR-624, miR-625, miR-626, miR-627, miR-628, miR-629, miR-630, miR-631, miR-632, miR-633, miR-634, miR-635, miR-636, miR-637, miR-638, miR-639, miR-640, miR-641, miR-642, miR-643, miR-644, miR-645, miR-646, miR-647, miR-648, miR-649, miR-650, miR-651, miR-652, miR-653, miR-654, miR-655, miR-656, miR-657, miR-658, miR-659, miR-660, miR-661, miR-662, miR-663, miR-7, miR-9, miR-9*, miR-92, miR-93, miR-95, miR-96, miR-98, miR-99a and miR-99b.
16. The method according to claim 13, characterized in that said evaluating the physiological and/or pathological condition of a subject is to determine the physiological and/or pathological condition of the subject after being administrated a test sample.
17. The method according to claim 16, characterized in that the method is useful for screening the test sample for the activities on the prevention and/or treatment of diseases.
18. The method according to claim 13, characterized in that said evaluating the physiological and/or pathological condition of a subject is to diagnose and/or differentially diagnose the diseases of the subject.
19. The method according to claim 13, characterized in that said evaluating the physiological and/or pathological condition of a subject is to evaluate the effectiveness of treating the diseases of the subject.
20. The method according to claim 13, characterized in that said evaluating the physiological and/or pathological condition of a subject is to predict the occurrence of diseases of the subject.
21. The method according to claim 20, characterized in that the occurrence of diseases is the occurrence of complications and/or the relapse of malignant diseases.
22. The method according to claim 17, characterized in that the diseases include various tumors; various acute and chronic infectious diseases e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS; bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute and chronic infectious diseases caused by various pathogenic microorganisms; other acute and chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular disease, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system.
23. The method according to claim 13, characterized in that the method is useful for detecting the subject for prohibited drugs-taking.
24. The method according to claim 13, characterized in that the method for determining all detectable microRNAs stably existing in serum/plasma of a subject is one or more selected from the group consisting of RT-PCR method, Real-time PCR method, Northern blotting method, RNase protection assay, Solexa sequencing technology and biochip method.
25. The method according to claim 24, characterized in that the method is RT-PCR method which includes the following steps:
- (1) extracting the total RNA from the serum/plasma of the subject, and obtaining cDNA samples by RNA reverse transcription reaction; or collecting serum/plasma samples from the subject and conducting reverse transcription reaction with serum/plasma being a buffer so as to prepare cDNA samples;
- (2) designing a primer by use of microRNAs and conducting PCR reaction;
- (3) conducting agarose gel electrophoresis of PCR products; and
- (4) observing agarose gel under ultraviolet Lamp after EB staining.
26. The method according to claim 24, characterized in that the method is Real-time PCR which includes the following steps:
- (1) extracting the total RNA from the serum/plasma of the subject, and obtaining cDNA samples by RNA reverse transcription reaction; or collecting serum/plasma samples from the subject, preparing cDNA samples by reverse transcription reaction with serum/plasma being a buffer;
- (2) designing a primer by use of microRNAs;
- (3) adding a fluorescent probe to conduct PCR reaction;
- (4) detecting and comparing the variation in levels of microRNAs in the serum/plasma samples relative to those of microRNAs in normal serum/plasma.
27. The method according to claim 13, characterized in that the serum/plasma derives from living bodies, tissues, organs and/or corpuses of the subject.
28. A kit for evaluating the physiological and/or pathological condition of a subject, wherein the kit comprises the tools useful for determining all detectable microRNAs stably existing in the serum/plasma of the subject.
29. The kit according to claim 28, characterized in that the kit comprises the primers of all mature microRNAs in human serum/plasma.
30. The kit according to claim 28, characterized in that the kit comprises the primers of let-7a, let-7b, let-7c, let-7d, let-7e, let-7f, let-7g, let-7i, miR-1, miR-100, miR-101, miR-103, miR-105, miR-106a, miR-106b, miR-107, miR-10a, miR-10b, miR-122a, miR-124a, miR-125a, miR-125b, miR-126, miR-126*, miR-127, miR-128a, miR-128b, miR-129, miR-130a, miR-130b, miR-132, miR-133a, miR-133b, miR-134, miR-135a, miR-135b, miR-136, miR-137, miR-138, miR-139, miR-140, miR-141, miR-142-3p, miR-142-5p, miR-143, miR-144, miR-145, miR-146a, miR-146b, miR-147, miR-148a, miR-148b, miR-149, miR-150, miR-151, miR-152, miR-153, miR-154, miR-154*, miR-155, miR-15a, miR-15b, miR-16, miR-17-3p, miR-17-5p, miR-181a, miR-181b, miR-181c, miR-181d, miR-182, miR-182*, miR-183, miR-184, miR-185, miR-186, miR-187, miR-188, miR-189, miR-18a, miR-18a*, miR-18b, miR-190, miR-191, miR-191*, miR-192, miR-193a, miR-193b, miR-194, miR-195, miR-196a, miR-196b, miR-197, miR-198, miR-199a, miR-199a*, miR-199b, miR-19a, miR-19b, miR-200a, miR-200a*, miR-200b, miR-200c, miR-202, miR-202*, miR-203, miR-204, miR-205, miR-206, miR-208, miR-20a, miR-20b, miR-21, miR-210, miR-211, miR-212, miR-213, miR-214, miR-215, miR-216, miR-217, miR-218, miR-219, miR-22, miR-220, miR-221, miR-222, miR-223, miR-224, miR-23a, miR-23b, miR-24, miR-25, miR-26a, miR-26b, miR-27a, miR-27b, miR-28, miR-296, miR-299-3p, miR-299-5p, miR-29a, miR-29b, miR-29c, miR-301, miR-302a, miR-302a*, miR-302b, miR-302b*, miR-302c, miR-302c*, miR-302d, miR-30a-3p, miR-30a-5p, miR-30b, miR-30c, miR-30d, miR-30e-3p, miR-30e-5p, miR-31, miR-32, miR-320, miR-323, miR-324-3p, miR-324-5p, miR-325, miR-326, miR-328, miR-329, miR-33, miR-330, miR-331, miR-335, miR-337, miR-338, miR-339, miR-33b, miR-340, miR-342, miR-345, miR-346, miR-34a, miR-34b, miR-34c, miR-361, miR-362, miR-363, miR-363*, miR-365, miR-367, miR-368, miR-369-3p, miR-369-5p, miR-370, miR-371, miR-372, miR-373, miR-373*, miR-374, miR-375, miR-376a, miR-376a*, miR-376b, miR-377, miR-378, miR-379, miR-380-3p, miR-380-5p, miR-381, miR-382, miR-383, miR-384, miR-409-3p, miR-409-5p, miR-410, miR-411, miR-412, miR-421, miR-422a, miR-422b, miR-423, miR-424, miR-425, miR-425-5p, miR-429, miR-431, miR-432, miR-432*, miR-433, miR-448, miR-449, miR-450, miR-451, miR-452, miR-452*, miR-453, miR-455, miR-483, miR-484, miR-485-3p, miR-485-5p, miR-486, miR-487a, miR-487b, miR-488, miR-489, miR-490, miR-491, miR-492, miR-493, miR-493-3p, miR-494, miR-495, miR-496, miR-497, miR-498, miR-499, miR-500, miR-501, miR-502, miR-503, miR-504, miR-505, miR-506, miR-507, miR-508, miR-509, miR-510, miR-511, miR-512-3p, miR-512-5p, miR-513, miR-514, miR-515-3p, miR-515-5p, miR-516-3p, miR-516-5p, miR-517*, miR-517a, miR-517b, miR-517c, miR-518a, miR-518a-2*, miR-518b, miR-518c, miR-518c*, miR-518d, miR-518e, miR-518f, miR-518f*, miR-519a, miR-519b, miR-519c, miR-519d, miR-519e, miR-519e*, miR-520a, miR-520a*, miR-520b, miR-520c, miR-520d, miR-520d*, miR-520e, miR-520f, miR-520g, miR-520h, miR-521, miR-522, miR-523, miR-524, miR-524*, miR-525, miR-525*, miR-526a, miR-526b, miR-526b*, miR-526c, miR-527, miR-532, miR-542-3p, miR-542-5p, miR-544, miR-545, miR-548a, miR-548b, miR-548c, miR-548d, miR-549, miR-550, miR-551a, miR-552, miR-553, miR-554, miR-555, miR-556, miR-557, miR-558, miR-559, miR-560, miR-561, miR-562, miR-563, miR-564, miR-565, miR-566, miR-567, miR-568, miR-569, miR-570, miR-571, miR-572, miR-573, miR-574, miR-575, miR-576, miR-577, miR-578, miR-579, miR-580, miR-581, miR-582, miR-583, miR-584, miR-585, miR-586, miR-587, miR-588, miR-589, miR-590, miR-591, miR-592, miR-593, miR-594, miR-595, miR-596, miR-597, miR-598, miR-599, miR-600, miR-601, miR-602, miR-603, miR-604, miR-605, miR-606, miR-607, miR-608, miR-609, miR-610, miR-611, miR-612, miR-613, miR-614, miR-615, miR-616, miR-617, miR-618, miR-619, miR-620, miR-621, miR-622, miR-623, miR-624, miR-625, miR-626, miR-627, miR-628, miR-629, miR-630, miR-631, miR-632, miR-633, miR-634, miR-635, miR-636, miR-637, miR-638, miR-639, miR-640, miR-641, miR-642, miR-643, miR-644, miR-645, miR-646, miR-647, miR-648, miR-649, miR-650, miR-651, miR-652, miR-653, miR-654, miR-655, miR-656, miR-657, miR-658, miR-659, miR-660, miR-661, miR-662, miR-663, miR-7, miR-9, miR-9*, miR-92, miR-93, miR-95, miR-96, miR-98, miR-99a and miR-99b.
31. The kit according to claim 28, characterized in that said evaluating the physiological and/or pathological condition of a subject is to determine the physiological and/or pathological condition of a subject after being administrated a test sample.
32. The kit according to claim 31, characterized in that the kit is useful for screening the test sample for the activities on the prevention and/or treatment of diseases.
33. The kit according to claim 28, characterized in that said evaluating the physiological and/or pathological condition of a subject is to diagnose and/or differentially diagnose the diseases of the subject.
34. The kit according to claim 28, characterized in that said evaluating the physiological and/or pathological condition of a subject is to evaluate the effectiveness of treating the diseases of the subject.
35. The kit according to claim 28, characterized in that said evaluating the physiological and/or pathological condition of a subject is to predict the occurrence of diseases of the subject.
36. The kit according to claim 35, characterized in that the occurrence of diseases is the occurrence of complications and/or the relapse of malignant diseases.
37. The kit according to claim 32, characterized in that the diseases include various tumors, various acute and chronic infectious diseases e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute and chronic infectious diseases caused by various pathogenic microorganisms; other acute and chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular disease, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system.
38. The kit according to claim 28, characterized in that the kit is useful for detecting the subject for prohibited drugs-taking.
39. The kit according to claim 28, characterized in that the serum/plasma of the subject are from living bodies, tissues, organs and/or corpuses of the subject.
40. A biochip for evaluating the physiological and/or pathological condition of a subject, wherein the biochip contains components useful for determining all detectable microRNAs stably existing in the serum/plasma of the subject.
41. The biochip according to claim 40, characterized in that the biochip contains the probes for all mature microRNAs in human serum/plasma.
42. The biochip according to claim 40, characterized in that the biochip comprises the following probes: Corre- sponding micro- Probes RNas Sequences of probes probe-let-7a let-7a AACTATACAACCTACTACCTCA probe-let-7b let-7b AACCACACAACCTACTACCTCA probe-let-7c let-7c AACCATACAACCTACTACCTCA probe-let-7d let-7d ACTATGCAACCTACTACCTCT probe-let-7e let-7e ACTATACAACCTCCTACCTCA probe-let-7f let-7f AACTATACAATCTACTACCTCA probe-let-7g let-7g ACTGTACAAACTACTACCTCA probe-let-7i let-7i ACAGCACAAACTACTACCTCA probe-miR-1 miR-1 TACATACTTCTTTACATTCCA probe-miR-100 miR-100 CACAAGTTCGGATCTACGGGTT probe-miR-101 miR-101 CTTCAGTTATCACAGTACTGTA probe-miR-103 miR-103 TCATAGCCCTGTACAATGCTGCT probe-miR-105 miR-105 ACAGGAGTCTGAGCATTTGA probe-miR-106a miR-106a GCTACCTGCACTGTAAGCACTTTT probe-miR-106b miR-106b ATCTGCACTGTCAGCACTTTA probe-miR-107 miR-107 TGATAGCCCTGTACAATGCTGCT probe-miR-10a miR-10a CACAAATTCGGATCTACAGGGTA probe-miR-10b miR-10b ACAAATTCGGTTCTACAGGGTA probe-miR-122a miR-122a ACAAACACCATTGTCACACTCCA probe-miR-124a miR-124a TGGCATTCACCGCGTGCCTTAA probe-miR-125a miR-125a CACAGGTTAAAGGGTCTCAGGGA probe-miR-125b miR-125b TCACAAGTTAGGGTCTCAGGGA probe-miR-126 miR-126 GCATTATTACTCACGGTACGA probe-miR-126* miR-126* CGCGTACCAAAAGTAATAATG probe-miR-127 miR-127 AGCCAAGCTCAGACGGATCCGA probe-miR-128a miR-128a AAAAGAGACCGGTTCACTGTGA probe-miR-128b miR-128b GAAAGAGACCGGTTCACTGTGA probe-miR-129 miR-129 GCAAGCCCAGACCGCAAAAAG probe-miR-130a miR-130a ATGCCCTTTTAACATTGCACTG probe-miR-130b miR-130b ATGCCCTTTCATCATTGCACTG probe-miR-132 miR-132 CGACCATGGCTGTAGACTGTTA probe-miR-133a miR-133a ACAGCTGGTTGAAGGGGACCAA probe-miR-133b miR-133b TAGCTGGTTGAAGGGGACCAA probe-miR-134 miR-134 CCCTCTGGTCAACCAGTCACA probe-miR-135a miR-135a TCACATAGGAATAAAAAGCCATA probe-miR-135b miR-135b CACATAGGAATGAAAAGCCATA probe-miR-136 miR-136 TCCATCATCAAAACAAATGGAGT probe-miR-137 miR-137 CTACGCGTATTCTTAAGCAATA probe-miR-138 miR-138 GATTCACAACACCAGCT probe-miR-139 miR-139 AGACACGTGCACTGTAGA probe-miR-140 miR-140 CTACCATAGGGTAAAACCACT probe-miR-141 miR-141 CCATCTTTACCAGACAGTGTTA probe-miR-142- miR-142- TCCATAAAGTAGGAAACACTACA 3p 3p probe-miR-142- miR-142- GTAGTGCTTTCTACTTTATG 5p 5p probe-miR-143 miR-143 TGAGCTACAGTGCTTCATCTCA probe-miR-144 miR-144 CTAGTACATCATCTATACTGTA probe-miR-145 miR-145 AAGGGATTCCTGGGAAAACTGGAC probe-miR-146a miR-146a AACCCATGGAATTCAGTTCTCA probe-miR-146b miR-146b AGCCTATGGAATTCAGTTCTCA probe-miR-147 miR-147 GCAGAAGCATTTCCACACAC probe-miR-148a miR-148a ACAAAGTTCTGTAGTGCACTGA probe-miR-148b miR-148b ACAAAGTTCTGTGATGCACTGA probe-miR-149 miR-149 GGAGTGAAGACACGGAGCCAGA probe-miR-150 miR-150 CACTGGTACAAGGGTTGGGAGA probe-miR-151 miR-151 CCTCAAGGAGCTTCAGTCTAGT probe-miR-152 miR-152 CCCAAGTTCTGTCATGCACTGA probe-miR-153 miR-153 TCACTTTTGTGACTATGCAA probe-miR-154 miR-154 CGAAGGCAACACGGATAACCTA probe-miR-154* miR-154* AATAGGTCAACCGTGTATGATT probe-miR-155 miR-155 CCCCTATCACGATTAGCATTAA probe-miR-15a miR-15a CACAAACCATTATGTGCTGCTA probe-miR-15b miR-15b TGTAAACCATGATGTGCTGCTA probe-miR-16 miR-16 CGCCAATATTTACGTGCTGCTA probe-miR-17- miR-17- ACAAGTGCCTTCACTGCAGT 3p 3p probe-miR-17- miR-17- ACTACCTGCACTGTAAGCACTTTG 5p 5p probe-miR-181a miR-181a ACTCACCGACAGCGTTGAATGTT probe-miR-181b miR-181b CCCACCGACAGCAATGAATGTT probe-miR-181c miR-181c ACTCACCGACAGGTTGAATGTT probe-miR-181d miR-181d AACCCACCGACAACAATGAATGTT probe-miR-182 miR-182 TGTGAGTTCTACCATTGCCAAA probe-miR-182* miR-182* TAGTTGGCAAGTCTAGAACCA probe-miR-183 miR-183 CAGTGAATTCTACCAGTGCCATA probe-miR-184 miR-184 ACCCTTATCAGTTCTCCGTCCA probe-miR-185 miR-185 GAACTGCCTTTCTCTCCA probe-miR-186 miR-186 AAGCCCAAAAGGAGAATTCTTTG probe-miR-187 miR-187 CGGCTGCAACACAAGACACGA probe-miR-188 miR-188 ACCCTCCACCATGCAAGGGATG probe-miR-189 miR-189 ACTGATATCAGCTCAGTAGGCAC probe-miR-18a miR-18a TATCTGCACTAGATGCACCTTA probe-miR-18a* miR-18a* AGAAGGAGCACTTAGGGCAGT probe-miR-18b miR-18b TAACTGCACTAGATGCACCTTA probe-miR-190 miR-190 ACCTAATATATCAAACATATCA probe-miR-191 miR-191 AGCTGCTTTTGGGATTCCGTTG probe-miR-191* miR-191* GGGGACGAAATCCAAGCGCAGC probe-miR-192 miR-192 GGCTGTCAATTCATAGGTCAG probe-miR-193a miR-193a CTGGGACTTTGTAGGCCAGTT probe-miR-193b miR-193b AAAGCGGGACTTTGAGGGCCAGTT probe-miR-194 miR-194 TCCACATGGAGTTGCTGTTACA probe-miR-195 miR-195 GCCAATATTTCTGTGCTGCTA probe-miR-196a miR-196a CCAACAACATGAAACTACCTA probe-miR-196b miR-196b CCAACAACAGGAAACTACCTA probe-miR-197 miR-197 GCTGGGTGGAGAAGGTGGTGAA probe-miR-198 miR-198 CCTATCTCCCCTCTGGACC probe-miR-199a miR-199a GAACAGGTAGTCTGAACACTGGG probe-miR- miR-199a* AACCAATGTGCAGACTACTGTA 199a* probe-miR-199b miR-199b GAACAGATAGTCTAAACACTGGG probe-miR-19a miR-19a TCAGTTTTGCATAGATTTGCACA probe-miR-19b miR-19b TCAGTTTTGCATGGATTTGCACA probe-miR-200a miR-200a ACATCGTTACCAGACAGTGTTA probe-miR- miR-200a* TCCAGCACTGTCCGGTAAGATG 200a* probe-miR-200b miR-200b GTCATCATTACCAGGCAGTATTA probe-miR-200c miR-200c CCATCATTACCCGGCAGTATTA probe-miR-202 miR-202 TTTTCCCATGCCCTATACCTCT probe-miR-202* miR-202* AAAGAAGTATATGCATAGGAAA probe-miR-203 miR-203 CTAGTGGTCCTAAACATTTCAC probe-miR-204 miR-204 AGGCATAGGATGACAAAGGGAA probe-miR-205 miR-205 CAGACTCCGGTGGAATGAAGGA probe-miR-206 miR-206 CCACACACTTCCTTACATTCCA probe-miR-208 miR-208 ACAAGCTTTTTGCTCGTCTTAT probe-miR-20a miR-20a CTACCTGCACTATAAGCACTTTA probe-miR-20b miR-20b CTACCTGCACTATGAGCACTTTG probe-miR-21 miR-21 TCAACATCAGTCTGATAAGCTA probe-miR-210 miR-210 TCAGCCGCTGTCACACGCACAG probe-miR-211 miR-211 AGGCGAAGGATGACAAAGGGAA probe-miR-212 miR-212 GGCCGTGACTGGAGACTGTTA probe-miR-213 miR-213 GGTACAATCAACGGTCGATGGT probe-miR-214 miR-214 CTGCCTGTCTGTGCCTGCTGT probe-miR-215 miR-215 GTCTGTCAATTCATAGGTCAT probe-miR-216 miR-216 CACAGTTGCCAGCTGAGATTA probe-miR-217 miR-217 ATCCAATCAGTTCCTGATGCAGTA probe-miR-218 miR-218 ACATGGTTAGATCAAGCACAA probe-miR-219 miR-219 AGAATTGCGTTTGGACAATCA probe-miR-22 miR-22 ACAGTTCTTCAACTGGCAGCTT probe-miR-220 miR-220 AAAGTGTCAGATACGGTGTGG probe-miR-221 miR-221 GAAACCCAGCAGACAATGTAGCT probe-miR-222 miR-222 GAGACCCAGTAGCCAGATGTAGCT probe-miR-223 miR-223 GGGGTATTTGACAAACTGACA probe-miR-224 miR-224 TAAACGGAACCACTAGTGACTTG probe-miR-23a miR-23a GGAAATCCCTGGCAATGTGAT probe-miR-23b miR-23b GGTAATCCCTGGCAATGTGAT probe-miR-24 miR-24 CTGTTCCTGCTGAACTGAGCCA probe-miR-25 miR-25 TCAGACCGAGACAAGTGCAATG probe-miR-26a miR-26a GCCTATCCTGGATTACTTGAA probe-miR-26b miR-26b AACCTATCCTGAATTACTTGAA probe-miR-27a miR-27a GCGGAACTTAGCCACTGTGAA probe-miR-27b miR-27b GCAGAACTTAGCCACTGTGAA probe-miR-28 miR-28 CTCAATAGACTGTGAGCTCCTT probe-miR-296 miR-296 ACAGGATTGAGGGGGGGCCCT probe-miR-299- miR-299- AAGCGGTTTACCATCCCACATA 3p 3p probe-miR-299- miR-299- ATGTATGTGGGACGGTAAACCA 5p 5p probe-miR-29a miR-29a AACCGATTTCAGATGGTGCTA probe-miR-29b miR-29b AACACTGATTTCAAATGGTGCTA probe-miR-29c miR-29c ACCGATTTCAAATGGTGCTA probe-miR-301 miR-301 GCTTTGACAATACTATTGCACTG probe-miR-302a miR-302a TCACCAAAACATGGAAGCACTTA probe-miR- miR-302a* AAAGCAAGTACATCCACGTTTA 302a probe-miR-302b miR-302b CTACTAAAACATGGAAGCACTTA probe-miR- miR-302b* AGAAAGCACTTCCATGTTAAAGT 302b* probe-miR-302c miR-302c CCACTGAAACATGGAAGCACTTA probe-miR- miR-302c* CAGCAGGTACCCCCATGTTAAA 302c* probe-miR-302d miR-302d ACACTCAAACATGGAAGCACTTA probe-miR-30a- miR-30a- GCTGCAAACATCCGACTGAAAG 3p 3p probe-miR-30a- miR-30a- CTTCCAGTCGAGGATGTTTACA 5p 5p probe-miR-30b miR-30b AGCTGAGTGTAGGATGTTTACA probe-miR-30c miR-30c GCTGAGAGTGTAGGATGTTTACA probe-miR-30d miR-30d CTTCCAGTCGGGGATGTTTACA probe-miR-30e- miR-30e- GCTGTAAACATCCGACTGAAAG 3p 3p probe-miR-30e- miR-30e- TCCAGTCAAGGATGTTTACA 5p 5p probe-miR-31 miR-31 CAGCTATGCCAGCATCTTGCC probe-miR-32 miR-32 GCAACTTAGTAATGTGCAATA probe-miR-320 miR-320 TTCGCCCTCTCAACCCAGCTTTT probe-miR-323 miR-323 AGAGGTCGACCGTGTAATGTGC probe-miR-324-3p miR-324- CCAGCAGCACCTGGGGCAGTGG 3p 3p probe-miR-324- miR-324- ACACCAATGCCCTAGGGGATGCG 5p 5p probe-miR-325 miR-325 ACACTTACTGGACACCTACTAGG probe-miR-326 miR-326 CTGGAGGAAGGGCCCAGAGG probe-miR-328 miR-328 ACGGAAGGGCAGAGAGGGCCAG probe-miR-329 miR-329 AAAGAGGTTAACCAGGTGTGTT probe-miR-33 miR-33 CAATGCAACTACAATGCAC probe-miR-330 miR-330 TCTCTGCAGGCCGTGTGCTTTGC probe-miR-331 miR-331 TTCTAGGATAGGCCCAGGGGC probe-miR-335 miR-335 ACATTTTTCGTTATTGCTCTTGA probe-miR-337 miR-337 AAAGGCATCATATAGGAGCTGGA probe-miR-338 miR-338 TCAACAAAATCACTGATGCTGGA probe-miR-339 miR-339 TGAGCTCCTGGAGGACAGGGA probe-miR-33b miR-33b TGCAATGCAACAGCAATGCAC probe-miR-340 miR-340 GGCTATAAAGTAACTGAGACGGA probe-miR-342 miR-342 GACGGGTGCGATTTCTGTGTGAGA probe-miR-345 miR-345 GCCCTGGACTAGGAGTCAGCA probe-miR-346 miR-346 AGAGGCAGGCATGCGGGCAGACA probe-miR-34a miR-34a AACAACCAGCTAAGACACTGCCA probe-miR-34b miR-34b CAATCAGCTAATGACACTGCCTA probe-miR-34c miR-34c GCAATCAGCTAACTACACTGCCT probe-miR-361 miR-361 GTACCCCTGGAGATTCTGATAA probe-miR-362 miR-362 CTCACACCTAGGTTCCAAGGATT probe-miR-363 miR-363 TTACAGATGGATACCGTGCAAT probe-miR-363* miR-363* AAATTGCATCGTGATCCACCCG probe-miR-365 miR-365 ATAAGGATTTTTAGGGGCATTA probe-miR-367 miR-367 TCACCATTGCTAAAGTGCAATT probe-miR-368 miR-368 AAACGTGGAATTTCCTCTATGT probe-miR-369- miR-369- AAAGATCAACCATGTATTATT 3p 3p probe-miR-369- miR-369- GCGAATATAACACGGTCGATCT 5p 5p probe-miR-370 miR-370 CCAGGTTCCACCCCAGCAGGC probe-miR-371 miR-371 ACACTCAAAAGATGGCGGCAC probe-miR-372 miR-372 ACGCTCAAATGTCGCAGCACTTT probe-miR-373 miR-373 ACACCCCAAAATCGAAGCACTTC probe-miR-373* miR-373* GGAAAGCGCCCCCATTTTGAGT probe-miR-374 miR-374 CACTTATCAGGTTGTATTATAA probe-miR-375 miR-375 TCACGCGAGCCGAACGAACAAA probe-miR-376a miR-376a ACGTGGATTTTCCTCTATGAT probe-miR- miR-376a* CTCATAGAAGGAGAATCTACC 376a* probe-miR-376b miR-376b AACATGGATTTTCCTCTATGAT probe-miR-377 miR-377 ACAAAAGTTGCCTTTGTGTGAT probe-miR-378 miR-378 ACACAGGACCTGGAGTCAGGAG probe-miR-379 miR-379 TACGTTCCATAGTCTACCA probe-miR-380- miR-380- AAGATGTGGACCATATTACATA 3p 3p probe-miR-380- miR-380- GCGCATGTTCTATGGTCAACCA 5p 5p probe-miR-381 miR-381 ACAGAGAGCTTGCCCTTGTATA probe-miR-382 miR-382 CGAATCCACCACGAACAACTTC probe-miR-383 miR-383 AGCCACAATCACCTTCTGATCT probe-miR-384 miR-384 TATGAACAATTTCTAGGAAT probe-miR-409- miR-409- AGGGGTTCACCGAGCAACATTCG 3p 3p probe-miR-409- miR-409- TGCAAAGTTGCTCGGGTAACCT 5p 5p probe-miR-410 miR-410 AACAGGCCATCTGTGTTATATT probe-miR-411 miR-411 CGTACGCTATACGGTCTACTA probe-miR-412 miR-412 ACGGCTAGTGGACCAGGTGAAGT probe-miR-421 miR-421 GCGCCCAATTAATGTCTGTTGAT probe-miR-422a miR-422a GGCCTTCTGACCCTAAGTCCAG probe-miR-422b miR-422b GGCCTTCTGACTCCAAGTCCAG probe-miR-423 miR-423 CTGAGGGGCCTCAGACCGAGCT probe-miR-424 miR-424 TTCAAAACATGAATTGCTGCTG probe-miR-425 miR-425 GGCGGACACGACATTCCCGAT probe-miR-425- miR-425- TCAACGGGAGTGATCGTGTCATT 5p 5p probe-miR-429 miR-429 ACGGTTTTACCAGACAGTATTA probe-miR-431 miR-431 TGCATGACGGCCTGCAAGACA probe-miR-432 miR-432 CCACCCAATGACCTACTCCAAGA nrobe-miR-432* miR-432* AGACATGGAGGAGCCATCCAG probe-miR-433 miR-433 ACACCGAGGAGCCCATCATGAT probe-miR-448 miR-448 ATGGGACATCCTACATATGCAA probe-miR-449 miR-449 ACCAGCTAACAATACACTGCCA probe-miR-450 miR-450 TATTAGGAACACATCGCAAAAA probe-miR-451 miR-451 AAACTCAGTAATGGTAACGGTTT probe-miR-452 miR-452 GTCTCAGTTTCCTCTGCAAACA probe-miR-452* miR-452* CTTCTTTGCAGATGAGACTGA probe-miR-453 miR-453 CGAACTCACCACGGACAACCTC probe-miR-455 miR-455 CGATGTAGTCCAAAGGCACATA probe-miR-483 miR-483 AGAAGACGGGAGGAGAGGAGTGA probe-miR-484 miR-484 ATCGGGAGGGGACTGAGCCTGA probe-miR-485- miR-485- AGAGGAGAGCCGTGTATGAC 3p 3p probe-miR-485- miR-485- GAATTCATCACGGCCAGCCTCT 5p 5p probe-miR-486 miR-486 CTCGGGGCAGCTCAGTACAGGA probe-miR-487a miR-487a AACTGGATGTCCCTGTATGATT probe-miR-487b miR-487b AAGTGGATGACCCTGTACGATT probe-miR-488 miR-488 TTGAGAGTGCCATTATCTGGG probe-miR-489 miR-489 GCTGCCGTATATGTGATGTCACT probe-miR-490 miR-490 CAGCATGGAGTCCTCCAGGTTG probe-miR-491 miR-491 TCCTCATGGAAGGGTTCCCCACT probe-miR-492 miR-492 AAGAATCTTGTCCCGCAGGTCCT probe-miR-493 miR-493 AATGAAAGCCTACCATGTACAA probe-miR-493- miR-493- CTGGCACACAGTAGACCTTCA 3p 3p probe-miR-494 miR-494 AAGAGGTTTCCCGTGTATGTTTCA probe-miR-495 miR-495 AAAGAAGTGCACCATGTTTGTTT probe-miR-496 miR-496 GAGATTGGCCATGTAAT probe-miR-497 miR-497 ACAAACCACAGTGTGCTGCTG probe-miR-498 miR-498 GAAAAACGCCCCCTGGCTTGAAA probe-miR-499 miR-499 TTAAACATCACTGCAAGTCTTAA probe-miR-500 miR-500 CAGAATCCTTGCCCAGGTGCAT probe-miR-501 miR-501 TCTCACCCAGGGACAAAGGATT probe-miR-502 miR-502 TAGCACCCAGATAGCAAGGAT probe-miR-503 miR-503 CTGCAGAACTGTTCCCGCTGCTA probe-miR-504 miR-504 ATAGAGTGCAGACCAGGGTCT probe-miR-505 miR-505 GAGGAAACCAGCAAGTGTTGAC probe-miR-506 miR-506 TCTACTCAGAAGGGTGCCTTA probe-miR-507 miR-507 TTCACTCCAAAAGGTGCAAAA probe-miR-508 miR-508 TCTACTCCAAAAGGCTACAATCA probe-miR-509 miR-509 TCTACCCACAGACGTACCAATCA probe-miR-510 miR-510 TGTGATTGCCACTCTCCTGAGTA probe-miR-511 miR-511 TGACTGCAGAGCAAAAGACAC probe-miR-512- miR-512- GACCTCAGCTATGACAGCACTT 3p 3p probe-miR-512- miR-512- GAAAGTGCCCTCAAGGCTGAGTG 5p 5p probe-miR-513 miR-513 ATAAATGACACCTCCCTGTGAA probe-miR-514 miR-514 CTACTCACAGAAGTGTCAAT probe-miR-515- miR-515- ACGCTCCAAAAGAAGGCACTC 3p 3p probe-miR-515- miR-515- CAGAAAGTGCTTTCTTTTGGAGAA 5p 5p probe-miR-516- miR-516- ACCCTCTGAAAGGAAGCA 3p 3p probe-miR-516- miR-516- AAAGTGCTTCTTACCTCCAGAT 5p 5p probe-miR-517* miR-517* AGACAGTGCTTCCATCTAGAGG probe-miR-517a miR-517a AACACTCTAAAGGGATGCACGAT probe-miR-517b miR-517b AACACTCTAAAGGGATGCACGA probe-miR-517c miR-517c ACACTCTAAAAGGATGCACGAT probe-miR-518a miR-518a TCCAGCAAAGGGAAGCGCTTT probe-miR- miR-518a- AAAGGGCTTCCCTTTGCAGA 518a-2* 2* probe-miR-518b miR-518b ACCTCTAAAGGGGAGCGCTTTG probe-miR-518c miR-518c CACTCTAAAGAGAAGCGCTTTG probe-miR- miR-518c* CAGAAAGTGCTTCCCTCCAGAGA 518c* probe-miR-518d miR-518d GCTCCAAAGGGAAGCGCTTTG probe-miR-518e miR-518e ACACTCTGAAGGGAAGCGCTTT probe-miR-518f miR-518f TCCTCTAAAGAGAAGCGCTTT probe-miR- miR-518f* AGAGAAAGTGCTTCCCTCTAGAG 518f* probe-miR-519a miR-519a GTAACACTCTAAAAGGATGCACTTT probe-miR-519b miR-519b AAACCTCTAAAAGGATGCACTTT probe-miR-519c miR-519c ATCCTCTAAAAAGATGCACTTT probe-miR-519d miR-519d ACACTCTAAAGGGAGGCACTTTG probe-miR-519e miR-519e ACACTCTAAAAGGAGGCACTTT probe-miR- miR-519e* GAAAGTGCTCCCTTTTGGAGAA 519e* probe-miR-520a miR-520a ACAGTCCAAAGGGAAGCACTTT probe-miR- miR-520a* AGAAAGTACTTCCCTCTGGAG 520a* probe-miR-520b miR-520b CCCTCTAAAAGGAAGCACTTT probe-miR-520c miR-520c AACCCTCTAAAAGGAAGCACTTT probe-miR-520d miR-520d AACCCACCAAAGAGAAGCACTTT probe-miR- miR-520d* CAGAAAGGGCTTCCCTTTGTAGA 520d* probe-miR-520e miR-520e CCCTCAAAAAGGAAGCACTTT probe-miR-520f miR-520f AACCCTCTAAAAGGAAGCACTT probe-miR-520g miR-520g ACACTCTAAAGGGAAGCACTTTGT probe-miR-520h miR-520h ACTCTAAAGGGAAGCACTTTGT probe-miR-521 miR-521 ACACTCTAAAGGGAAGTGCGTT probe-miR-522 miR-522 AACACTCTAAAGGGAACCATTTT probe-miR-523 miR-523 CCCTCTATAGGGAAGCGCGTT probe-miR-524 miR-524 ACTCCAAAGGGAAGCGCCTTC probe-miR-524* miR-524* GAGAAAGTGCTTCCCTTTGTAG probe-miR-525 miR-525 AGAAAGTGCATCCCTCTGGAG probe-miR-525* miR-525* GCTCTAAAGGGAAGCGCCTTC probe-miR-526a miR-526a AGAAAGTGCTTCCCTCTAGAG probe-miR-526b miR-526b AACAGAAAGTGCTTCCCTCAAGAG probe-miR- miR-526b* GCCTCTAAAAGGAAGCACTTT 526b* probe-miR-526c miR-526c AACAGAAAGCGCTTCCCTCTAGAG probe-miR-527 miR-527 AGAAAGGGCTTCCCTTTGCAG probe-miR-532 miR-532 ACGGTCCTACACTCAAGGCATG probe-miR-542- miR-542- TTTCAGTTATCAATCTGTCACA 3p 3p probe-miR-542- miR-542- CTCGTGACATGATGATCCCCGA 5p 5p probe-miR-544 miR-544 ACTTGCTAAAAATGCAGAAT probe-miR-545 miR-545 CACACAATAAATGTTTGCTGAT probe-miR-548a miR-548a GCAAAAGTAATTGCCAGTTTTG probe-miR-548b miR-548b ACAAAAGCAACTGAGGTTCTTG probe-miR-548c miR-548c GCAAAAGTAATTGAGATTTTTG probe-miR-548d miR-548d GCAAAAGAAACTGTGGTTTTTG probe-miR-549 miR-549 AGAGCTCATCCATAGTTGTCA probe-miR-550 miR-550 ATGTGCCTGAGGGAGTAAGACA probe-miR-551a miR-551a TGGAAACCAAGAGTGGGTCGC probe-miR-552 miR-552 TTGTCTAACCAGTCACCTGTT probe-miR-553 miR-553 AAAACAAAATCTCACCGTTTT probe-miR-554 miR-554 ACTGGCTGAGTCAGGACTAGC probe-miR-555 miR-555 ATCAGAGGTTCAGCTTACCCT probe-miR-556 miR-556 CATATTACAATGAGCTCATC probe-miR-557 miR-557 AGACAAGGCCCACCCGTGCAAAC probe-miR-558 miR-558 ATTTTGGTACAGCAGCTCA probe-miR-559 miR-559 TTTTGGTGCATATTTACTTTA probe-miR-560 miR-560 GGCGGCCGGCCGGCGCACGC probe-miR-561 miR-561 ACTTCAAGGATCTTAAACTTTG probe-miR-562 miR-562 GCAAATGGTACAGCTACTTT probe-miR-563 miR-563 GGGAAACGTATGTCAACCT probe-miR-564 miR-564 GCCTGCTGACACCGTGCCT probe-miR-565 miR-565 AAACAGACATCGCGAGCCAGCC probe-miR-566 miR-566 GTTGGGATCACAGGCGCCC probe-miR-567 miR-567 GTTCTGTCCTGGAAGAACATACT probe-miR-568 miR-568 GTGTGTATACATTTATACAT probe-miR-569 miR-569 ACTTTCCAGGATTCATTAACT probe-miR-570 miR-570 TGCAAAGGTAATTGCTGTTTTC probe-miR-571 miR-571 CTCACTCAGATGGCCAACTCA probe-miR-572 miR-572 TGGGCCACCGCCGAGCGGAC probe-miR-573 miR-573 CTGATCAGTTACACATCACTTCAG probe-miR-574 miR-574 GTGGGTGTGTGCATGAGCGTG probe-miR-575 miR-575 GCTCCTGTCCAACTGGCTC probe-miR-576 miR-576 CAAAGACGTGGAGAAATTAGAAT probe-miR-577 miR-577 CAGGTACCAATATTTTATCTA probe-miR-578 miR-578 ACAATCCTAGAGCACAAGAAG probe-miR-579 miR-579 ATCGCGGTTTATACCAAATGAAT probe-miR-580 miR-580 CCTAATGATTCATCATTCTCAA probe-miR-581 miR-581 ACTGATCTAGAGAACACAAGA probe-miR-582 miR-582 AGTAACTGGTTGAACAACTGTAA probe-miR-583 miR-583 GTAATGGGACCTTCCTCTTTG probe-miR-584 miR-584 CTCAGTCCCAGGCAAACCATAA probe-miR-585 miR-585 TAGCATACAGATACGCCCA probe-miR-586 miR-586 GGACCTAAAAATACAATGCATA probe-miR-587 miR-587 GTGACTCATCACCTATGGAAA probe-miR-588 miR-588 GTTCTAACCCATTGTGGCCAA probe-miR-589 miR-589 TCTGGGAACCGGCATTTGTTCTGA probe-miR-590 miR-590 CTGCACTTTTATGAATAAGCTC probe-miR-591 miR-591 ACAATGAGAACCCATGGTCT probe-miR-592 miR-592 ACATCATCGCATATTGACACAA probe-miR-593 miR-593 GCTGAGCAATGCCTGGCTGGTGCCT probe-miR-594 miR-594 AAAGTCACAGGCCACCCCAGATGGG probe-miR-595 miR-595 AGACACACCACGGCACACTTC probe-miR-596 miR-596 CCCGAGGAGCCGGGCAGGCTT probe-miR-597 miR-597 ACAGTGGTCATCGAGTGACACA probe-miR-598 miR-598 TGACGATGACAACGATGACGTA probe-miR-599 miR-599 GTTTGATAAACTGACACAAC probe-miR-600 miR-600 GAGCAAGGCTCTTGTCTGTAAGT probe-miR-601 miR-601 CTCCTCCAACAATCCTAGACCA probe-miR-602 miR-602 GGGCCGCAGCTGTCGCCCGTGTC probe-miR-603 miR-603 GCAAAAGTAATTGCAGTGTGTG probe-miR-604 miR-604 GTCCTGAATTCCGCAGCCT probe-miR-605 miR-605 AGGAGAAGGCACCATGGGATTTA probe-miR-606 miR-606 ATCTTTGATTTTCAGTAGTTT probe-miR-607 miR-607 GTTATAGATCTGGATTTGAAC probe-miR-608 miR-608 ACGGAGCTGTCCCAACACCACCCCT probe-miR-609 miR-609 AGAGATGAGAGAAACACCCT probe-miR-610 miR-610 TCCCAGCACACATTTAGCTCA probe-miR-611 miR-611 GTCAGACCCCGAGGGGTCCTCGC probe-miR-612 miR-612 AAGGAGCTCAGAAGCCCTGCCCAGC probe-miR-613 miR-613 GGCAAAGAAGGAACATTCCT probe-miR-614 miR-614 CCACCTGGCAAGAACAGGCGTTC probe-miR-615 miR-615 AGAGGGAGACCCAGGCTCGGA probe-miR-616 miR-616 AAGTCACTGAAGGGTTTTGAGT probe-miR-617 miR-617 GCCACCTTCAAATGGGAAGTCT probe-miR-618 miR-618 ACTCAGAAGGACAAGTAGAGTTT probe-miR-619 miR-619 ACTGGGCACAAACATGTCCAGGTC probe-miR-620 miR-620 ATTTCTATATCTATCTCCAT probe-miR-621 miR-621 AGGTAAGCGCTGTTGCTAGCC probe-miR-622 miR-622 GCTCCAACCTCAGCAGACTGT probe-miR-623 miR-623 ACCCAACAGCCCCTGCAAGGGAT probe-miR-624 miR-624 TGAACACAAGGTACTGGTACTA probe-miR-625 miR-625 AGGACTATAGAACTTTCCCCCT probe-miR-626 miR-626 AAGACATTTTCAGACAGCT probe-miR-627 miR-627 TCCTCTTTTCTTAGAGACTCAC probe-miR-628 miR-628 CGACTGCCACTCTTACTAGA probe-miR-629 miR-629 GCTGGGCTTACGTTGGGAGAAC probe-miR-630 miR-630 ACCTTCCCTGGTACAGAATACT probe-miR-631 miR-631 GCTGAGGTCTGGGCCAGGTCT probe-miR-632 miR-632 TCCCACAGGAAGCAGACAC probe-miR-633 miR-633 TTTATTGTGGTAGATACTATTAG probe-miR-634 miR-634 GTCCAAAGTTGGGGTGCTGGTT probe-miR-635 miR-635 GGACATTGTTTCAGTGCCCAAGT probe-miR-636 miR-636 CTGCGGGCGGGACGAGCAAGCACA probe-miR-637 miR-637 ACGCAGAGCCCGAAAGCCCCCAGT probe-miR-638 miR-638 AGGCCGCCACCCGCCCGCGATCCCT probe-miR-639 miR-639 ACAGCGCTCGCAACCGCAGCGAT probe-miR-640 miR-640 AGAGGCAGGTTCCTGGATCAT probe-miR-641 miR-641 GAGGTGACTCTATCCTATGTCTTT probe-miR-642 miR-642 CAAGACACATTTGGAGAGGGAC probe-miR-643 miR-643 CTACCTGAGCTAGCATACAAGT probe-miR-644 miR-644 GCTCTAAGAAAGCCACACT probe-miR-645 miR-645 TCAGCAGTACCAGCCTAGA probe-miR-646 miR-646 GCCTCAGAGGCAGCTGCTT probe-miR-647 miR-647 GAAGGAAGTGAGTGCAGCCAC probe-miR-648 miR-648 ACCAGTGCCCTGCACACTT probe-miR-649 miR-649 GACTCTTGAACAACACAGGTTT probe-miR-650 miR-650 GTCCTGAGAGCGCTGCCTCCT probe-miR-651 miR-651 CAAAAGTCAAGCTTATCCTAAA probe-miR-652 miR-652 TGCACAACCCTAGTGGCGCCATT probe-miR-653 miR-653 GTTCAGTAGAGATTGTTTCAA probe-miR-654 miR-654 GCACATGTTCTGCGGCCCACCA probe-miR-655 miR-655 AAAGAGGTTAACCATGTATTAT probe-miR-656 miR-656 AGAGGTTGACTGTATAATATT probe-miR-657 miR-657 CCTAGAGAGGGTGAGAACCTGCC probe-miR-658 miR-658 ACCAACGGACCTACTTCCCTCCGCC probe-miR-659 miR-659 TGGGGACCCTCCCTGAACCAAG probe-miR-660 miR-660 CAACTCCGATATGCAATGGGTA probe-miR-661 miR-661 ACGCGCAGGCCAGAGACCCAGGCA probe-miR-662 miR-662 CTGCTGGGCCACAACGTGGGA probe-miR-663 miR-663 GCGGTCCCGCGGCGCCCCGCCT probe-miR-7 miR-7 CAACAAAATCACTAGTCTTCCA probe-miR-9 miR-9 TCATACAGCTAGATAACCAAAGA probe-miR-9* miR-9* ACTTTCGGTTATCTAGCTTTA probe-miR-92 miR-92 CAGGCCGGGACAAGTGCAATA probe-miR-93 miR-93 CTACCTGCACGAACAGCACTTT probe-miR-95 miR-95 TGCTCAATAAATACCCGTTGAA probe-miR-96 miR-96 GCAAAAATGTGCTAGTGCCAAA probe-miR-98 miR-98 AACAATACAACTTACTACCTCA probe-miR-99a miR-99a CACAAGATCGGATCTACGGGTT probe-miR-99b miR-99b CGCAAGGTCGGTTCTACGGGTG
43. The biochip according to claim 40, characterized in that said evaluating the physiological and/or pathological condition of a subject is to determine the physiological and/or pathological condition of the subject after being administrated a test sample.
44. The biochip according to claims 43, characterized in that the biochip are useful for screening the test sample for the activities on the prevention and/or treatment of diseases.
45. The biochip according to claim 40, characterized in that said evaluating the physiological and/or pathological condition of a subject is to diagnose and/or differentially diagnose the diseases of the subject.
46. The biochip according to claim 40, characterized in that said evaluating the physiological and/or pathological condition of a subject is to evaluate the effectiveness of treating the diseases of the subject.
47. The biochip according to claim 40, characterized in that said evaluating the physiological and/or pathological condition of a subject is to predict the occurrence of diseases of the subject.
48. The biochip according to claim 47, characterized in that the occurrence of diseases is the occurrence of complications and/or the relapse of malignant diseases.
49. The biochip according to claim 44, characterized in that the diseases include various tumors, various acute and chronic infectious diseases e.g. viral diseases such as viral influenza, viral hepatitis, AIDS, SARS, bacterial diseases such as tuberculosis, bacterial pneumonia, and other acute and chronic infectious diseases caused by various pathogenic microorganisms; other acute and chronic diseases such as diseases of respiratory system, diseases of immune system, diseases of blood and hematopoietic system, diseases of circulatory system such as cardio-cerebrovascular disease, metabolic diseases of endocrine system, diseases of digestive system, diseases of nervous system, diseases of urinary system, diseases of reproductive system and diseases of locomotor system.
50. The biochip according to claim 40, characterized, in that the biochip are useful for detecting the subject for prohibited drugs-taking.
51. The chip according to claim 40, characterized in that the serum/plasma the subject is from living bodies, tissues, organs and/or corpuses of the subject.
Type: Application
Filed: Dec 6, 2007
Publication Date: Jul 8, 2010
Inventors: Chenyu Zhang (Jiangsu), Junfeng Zhang (Jiangsu), Xi Chen (Jiangsu), Yi Ba (Tianjin), Jiangning Chen (Jiangsu), Jin Wang (Jiangsu), Ke Zeng (Jiangsu), Hongjie Zhang (Jiangsu)
Application Number: 12/302,196
International Classification: C12Q 1/68 (20060101); C12M 1/34 (20060101);