METHOD OF MEASURING THE AFFINITY OF BIOMOLECULES
The invention provides a method of measuring the affinity of first and second biomolecules in which a first biomolecule is tethered by a first tether portion having a first tether portion length and a second biomolecule is tethered by a second tether portion having a second tether portion length, the method comprising determining binding of adjacent first and second biomolecules to each other, varying at least one of the first and second tether lengths and determining binding of the first and second biomolecules. The invention also provides apparatus suitable for use in the method of the invention.
This patent application is a divisional patent application of U.S. patent application Ser. No. 14/222,122, filed Mar. 21, 2014, which is a divisional patent application of U.S. patent application Ser. No. 12/094,073, filed Sep. 9, 2008, now U.S. Pat. No. 8,778,697, which is a National Stage Filing of PCT/GB2006/004208, filed Nov. 10, 2006, which claims priority to GB 05233663, filed Nov. 16, 2005, the disclosures of each of which are hereby incorporated in their entirety.
FIELD OF THE INVENTIONThis invention relates particularly, though not exclusively, to the field of analysis of biochemical pathways and to the interaction between biomolecules such as proteins and polypeptides.
BACKGROUND OF THE INVENTIONThere has been an explosion of biological information in the last few years resulting from the use of high throughput experimental techniques. These techniques range from genome sequencing, microarray analysis, yeast 2-hybrid protein-protein interaction assays, to RNAi screens and the use of automated image analysis to study cell biological processes.
Following the successful implementation of each ‘-omic’ technique, opportunities and bottlenecks are created at the interface between one set of techniques and the next. One key bottleneck is that of biochemistry.
Molecular machines, formed from complexes of proteins, are the building blocks underlying most cellular processes. Techniques such as the yeast 2-hybrid technique have been used to identify binary interactions between pairs of proteins on a genome-wide scale, while complementary analyses using complex purification and mass spectrometry are starting to identify the combinations of components that comprise each molecular machine. However, the detailed study of biochemical interactions requires the identification of affinity binding and rate constants, together with techniques for studying how these properties are physiologically regulated.
Standard ‘test tube’ biochemical techniques, including calorimetry and fluorescence anisotropy, require the time-consuming production and purification of microgram to milligram quantities of soluble proteins and are therefore unlikely to be scaled-up for high throughput applications. A potentially more promising technique, Surface Plasmon Resonance (Biacore®) requires somewhat less protein and can tolerate the presence of impurities (in some formats), but requires the careful timed flow of assay protein, followed by wash solutions over an immobilized binding partner and is therefore unlikely to be easily adapted for high throughput analyses. Typical protein requirements for Surface Plasmon Resonance and calorimetry are described below:
Isothermal Titration calorimetry:
Measures: Kd, Stoichiometry (n), ΔG, ΔN
Requires: 1 ml of 10 μM solution; 20 nMoles; 1 mg of 50 KDa protein.
Surface Plasmon Resonance (Biacore®)Measures: Kon, Koff, Kd
Requires: 2 mls of 100 nM solution; 200 pMoles; 10 μg of 50 KDa protein*.
* Calculation based on typical series of experiments required to establish a binding affinity in the ˜10 nM range.
The high levels of proteins that are required in these assays result from the requirement to ‘saturate’ binding ligand concentrations 4-10× higher than the dissociation constant. This imposes the typical requirements shown in Table 1.
These levels of protein require time consuming and relatively expensive conventional protein synthesis and purification systems.
In vitro translation ‘pull-down’ experiments can be used to identify binding interactions between small amounts of radiolabelled protein produced in a translation extract (100-150 ng produced). However, like the yeast 2-hybrid technique, they suffer from the disadvantage that they are non-quantitative, they screen for picomolar to low nanomolar ranges of affinities and fail to screen for lower affinity interactions.
There is a requirement for new high-throughput biochemical techniques that are quantitative, sensitive, may use small volumes of analyte, may require a low number of moles of analyte, may achieve high (up to mid-micromolar typically about 1-5 pM to about 10-20 μM) concentrations and may be adaptable for massively parallel analyses.
SUMMARY OF THE INVENTIONAccording to one aspect of the invention there is provided a method of measuring the affinity of first and second biomolecules in which a first biomolecule is tethered by a first tether portion having a first tether portion length and a second biomolecule is tethered by a second tether portion having a second tether portion length, determining binding of adjacent first and second biomolecules to each other, varying at least one of the first and second tether portion lengths and determining binding of the first and second biomolecules.
The method of the invention is advantageous in that it allows very accurate control of the concentration of amounts of biomolecules and also in that it needs only very small amounts of the biomolecules—it allows equilibrium-binding studies to be carried out in pico- to attolitre volumes. The low volumes allow a range of concentration-dependent biochemical assays to be performed with very low input amounts of each biomolecule. By way of example, in a theoretical determination comparing a method in accordance with the invention with conventional techniques, conventional calorimetry would require 20 nanomoles of protein or 1 mg of protein of a 50 KDa protein; Surface Plasmon Resonance would require 200 picomoles of protein corresponding to 10 micrograms for a 50 KDa protein. In contrast, a comparable method in accordance with the invention would require only 10 attomoles and 50 picograms for a 50 KDa protein. Typically, nano- to zeptolitre, preferably pico- to attolitre, volumes of first and/or second biomolecules are used.
In this context, the term “biomolecule” includes both naturally-occurring molecules and synthetic molecules.
The first and second biomolecules may be tethered to a solid support such as a glass slide or microbead. In one such configuration, the first and second biomolecules are separately tethered to the same solid support. Alternatively, the first and second biomolecules may be tethered together in a “Y-shaped” arrangement. In another embodiment, the first and second biomolecules may be joined by a tether but not tethered to a solid support, in a “linear molecule” arrangement. For example, the first and second biomolecules may be tethered together and present in a solution.
Where the biomolecules are tethered to a solid support, the biomolecules may be randomly arranged over the solid support. Alternatively, the biomolecules may be tethered to discrete portions of, or areas defined on, the solid support such that the first and second biomolecules can only interact if they “stretch” to span the gap between the discrete portions. By controlling the distance between the discrete portions and/or the tether length, the proportion of bound and free biomolecules may be altered allowing the determination of affinity described above. Discrete portions of the surface may be coupled to the first and second biomolecules using a range of techniques including photo, electron or ion beam lithography to sequentially deprotect portions for coupling. Alternatively, direct etching/modification using atomic force microscope tips may be used to introduce selective regional surface modification. An advantage of this type of approach is that inter-molecular distances may be directly controlled rather than relying on mean distances. In principle, this should allow for more accurate control of biomolecule concentration.
In a preferred embodiment where first and second biomolecules are tethered to a solid support, the method may be arranged to be operated in a nano-scale reaction zone. The formation of the reaction zone may be achieved by anchoring the tethers near each other so that at least some of the first and second biomolecules are closely adjacent to each other, such that the substantially hemispherical swept volumes defined by the free ends of each biomolecule overlap, allowing the first and second biomolecules to bind to each other. The volume of each hemispherical volume may be of the order of 2×103 to 1×1012 nm3. By varying the length of the tether portions, the effective concentrations of the biomolecules can be controlled allowing quantitative analyses.
The stiffness of the tethers is considered in terms of the persistence length (P) which is an experimentally measured parameter that characterises the stiffness as a single bending parameter of a flexible rod. (Bustamante, C., J. F. et al 1994. Science. 265:1599-1600; and Marko, J. F., and E. D. Siggia. 1995. Stretching DNA. Macromolecules. 28:8759-8770). In the case of relatively long tethers (P>approx five times less than the contour length of the tether) made of polymers such as DNA in solution, the tether can be represented by a worm-like chain model that is characterised by, the persistence length (P). Molecules much longer than the persistence length (P equals approx 50-90 nm for dsDNA) behave like random coils of a freely jointed chain with a segment length 2P and a Gaussian distribution of segment density.
In addition to varying the length of the tethers, the inter-anchor distance can be altered to vary the overlap of the swept volumes. This method can be used to alter the stoichiometry of tethered molecules and to fully exploit the special case when long flexible tethers are used.
Computer simulations (Monte Carlo) have been used to calculate the probabilities of free DNA end distribution (for example, see Jian and Vologodskii (1997). A combined wormlike-chain and bead model for dynamic simulations of long linear DNA, J. Comp. Physics 136 pp 168-179.).
The probability distribution of the free end of a tether in the nanotether context is determined by a number of factors including the stiffness of the tether, the temperature and the ionic conditions. By using long tethers in proportion to the persistence length (e.g. greater than 5 times P), the inter-anchor distance can be varied to probe the effective concentration gradient within the substantially hemispherical swept volume.
In this concentration gradient, the lowest concentration would be closest to the surface swept by the tether at its full contour length (stretched straight). The concentration would then increase to a maximum close to the average centre of mass due to entropic considerations. The probability that two tethered biomolecules will interact at a particular inter-anchor distance will thus be dependent on the calculated probability distribution and will increase as the inter-anchor distance decreases. Approaches to alter the probability distribution of flexible tethers within their swept volumes (e.g. inducing bulk liquid flow or the use of vibrating supports) may be used to enhance the utility of tethers far beyond their persistence lengths (e.g. 20-40 times P).
By measuring the interaction distributions of a range of ‘test case’ biomolecule interactions (e.g. GSK-3 and Axin peptide; streptavidin—biotin; antibody—antigen), it will be possible to correlate the probability distribution with the inter-anchor distance and to equate this directly to an affinity binding constant. Alternatively mathematical models of this process can also be produced based on the studies of Jian (supra).
Both varying tether length and inter-anchor distance are proposed as methods for varying tethered biomolecule concentrations. At high length: P values, the probability distribution may be the most effective method of calculating affinity. In a linear molecule or Y-shaped molecule embodiment, the first and second tether portion length may be varied to vary the biomolecule concentrations.
Techniques that measure the proportion of the first and second biomolecules that are molecularly close to each other can be used to quantify the proportion of interacting first and second biomolecules. For example, the proportion of first and second biomolecules that are molecularly close to each other can be determined by Forster resonance energy transfer (FRET).
In a preferred method, the assay readout is the intensity of FRET between fluorophores coupled to the head oligonucleotides attached to the first and second biomolecules. A laser, appropriate to the excitation maximum for a fluorophore attached to the first biomolecule, is used to excite that fluorophore. Emission at the wavelength maximum from a fluorophore attached to the second biomolecule is recorded to assess the level of FRET. In practice, for FRET to occur, an excited molecule of the first fluorophore has to be molecularly close (<10 nm) to the second fluorophore for energy to be transferred, leading to emission at the characteristic wavelength of the second fluorophore. This will occur when the first and second biomolecules are also molecularly close due to the formation of the first biomolecule/second biomolecule complexes. In a preferred variant of the FRET technique, fluorescence lifetime measurement (FRET/FLIM) is used to measure the time dependence of FRET since this technique offers improved sensitivity (‘Fluorescence Lifetime Imaging: An emerging technique in Fluorescence Microscopy’, C. G. Morgan, Chromosome Research, 4(4), 261-263, 1996.). Appropriate controls (e.g. spots of the first and second biomolecules alone) will be used to normalise signal levels.
In a preferred embodiment, FRET may be measured using a lens to focus the lasers on glass slides containing arrays of tethered biomolecules. In other embodiments, purpose-built machines are arranged to overcome the limitations that confocal microscopes have due to their design for other purposes. In particular, the use of photomultipliers and cooled charge-coupled devices (CCDs) may enhance the sensitivity of detection of the low level FRET signals, potentially leading to the detection of FRET between tethered pairs of single first and second biomolecules (for example, see Walter et al., Biopolymers (Nucleic Acid Sciences), Vol. 61, 224-241 (2002)). Alternatively, Total Internal Reflection Fluorescence Microscopy (TIRF) may be used (Surface fluorescence microscopy with evanescent illumination., Axelrod, D., Light Microscopy in Biology, Lacey, A. (ed), Oxford University Press, New York, 399-423 (1999)).
In an alternative solution, nanoscale spheres or “quantum dots”, nanocrystals which absorb light but quickly re-emit the light in a different colour, may be tethered in place of the single fluorophores. These conjugates may offer higher FRET efficiencies due to the increased number of fluorescent molecules. Alternatively, the nanoscale spheres would allow fluorescence correlation spectroscopy to be performed using a high-resolution light confocal microscope. For tethers longer than 2 Kb (0.6 μM), the formation of first biomolecule/second biomolecule complexes may be directly recorded due to the proportion of fluorescent dot pairs in proportion to those that show some separation.
The first and/or second tethers, or a single tether in the case of a linear molecule, may be formed from nucleotides. Preferably, a tether is generated from double stranded DNA (dsDNA). Alternatively, a tether may be made from other polymers such as carbon nanotubes (D. H. Jung et al Covalent attachment and hybridization of DNA oligonucleotides on patterned single-walled carbon nanotube films. Langmuir. 2004 Sep. 28; 20(20):8886-91.), amyloid fibrils, or DNA crossover complexes for example DX hybrids, which include an even number (typically 4, 6, or 8) strands of DNA and are somewhat stiffer than dsDNA; J. Am. Chem. Soc. (2000), 122, 1848-1860, Construction, Analysis, Ligation, and Self-Assembly of DNA Triple Crossover Complexes). Furthermore, the ‘stiffness’ or persistence length (P) and electrostatic charge of tethers such as dsDNA may be modulated by chemical modification, interchelation with molecules such as ethidium bromide or other suitable interchelating agents, which are typically organic compounds to allow insertion between the dsDNA bases or are positively charged and polymeric to complex with DNA based on affinity for the negatively charged phosphate backbone of DNA. The stiffness of DNA may also be altered by complexing with DNA binding proteins along the length of the tether. The stiffness of other tethers may be modulated by other means. For example, the stiffness of tethers comprising DX hybrids may be modulated by varying the number of strands; for tethers comprising carbon nanotubes by increasing the number of concentric tubes forming each nanotube.
In a preferred embodiment, variable-length dsDNA tether portions are ligated together to form a tether. For example, a tether body portion may be linked to head and tail tether portions to produce the tether. The nucleotides of the body portion may be ligated to head and tail portions in solution.
For non-nucleotide tethers, chemical cross-linking methods can be used to attach head and tail oligonucleotide linkers to the respective ends of the body portions of the tethers.
Where the tethers comprise nucleotides, the or each tether portion length may typically be of the order of 50 basepairs (bp) to 50 Kb preferably, 200 base pairs to 20 kbase pairs, or 30 to 12 000 nm, preferably 60 to 6000 nm, for other tethers.
The tethers may be tethered to a surface by means of anchors. The anchors may be single-stranded amino-modified oligonucleotides. The tethers (head, body and tail) can then be hybridised to a solid support to which anchor oligonucleotides have been immobilised. The solid support may be a modified glass substrate. Standard techniques may be used to covalently couple an anchor oligonucleotide (for example, see: Chrisey, L. A., Lee, G. U., and O'Ferrall, E. (1996) Covalent attachment of synthetic DNA to self-assembled monolayer films Nucleic Acids Res. 24:3031-3039). A preferred method involves coupling amino-modified anchor oligonucleotides to a glass support treated with an agent such as amino silane and p-phenylene1,4 diisothiocyanate (PDC). Other substrates that can be modified to bind a tether to a surface are also contemplated, including agarose and sepharose.
In one embodiment, the format of the support is a glass slide onto which oligonucleotide anchors or tethers are printed in arrays of spots using commercially available split pin arraying machines such as those available from Genetix. More specialist solid supports, based on miniaturisation techniques derived from microelectronics, may be used in more sophisticated implementations that are designed to further miniaturise the analysis and to integrate better with readout systems.
In an alternative format, the support may be provided by microbeads that are coupled in formats that generate a unique relationship between a single bead and tether combination. This format enables the adaptation of the technology to microfluidic systems, and may enhance probe density particularly where relatively long tethers, say about 50 μm, are used to test for high affinity interactions at high inter-anchor distances. Suitable microbeads may include polystyrene, coated ferrous/ferric particles, gold particles, sepharose, agarose, glass or carbon.
In an arrayed-spot implementation, amino-terminal oligonucleotide anchors for the first and second biomolecules may be covalently coupled to the modified glass substrate. A range of other approaches can be used to vary the inter-tether distance. In one implementation, the distance between the oligonucleotide anchors is increased by the use of a non-specific amino terminal oligonucleotide (which is designed not to bind to other tether components) that is titrated into the specific oligonucleotide mix. The greater the proportion of the non-specific oligonucleotide; the greater the resulting distance between specific oligonucleotide anchor. Alternatively, the proportion of modified silane molecules may be reduced prior to oligonucleotide coupling. Inter-anchor mean distances may be varied from distances greater than the tether length to the maximal oligonucleotide tether capacity. The maximal coupling density possible using published protocols (e.g. Chrisey et al 1996 supra) is 20 pmoles of bound DNA/cm2 which equates to an mean inter-anchor spacing of 1.6 nm; Chrisey, L. A., et al (1996) supra. This inter-anchor density massively exceeds that required for the most probable range of anchor densities which would normally range from about 5 nm to about 1 μm.
In the above implementation, the non-specific amino-specific oligonucleotide functions to cap the reactive groups and will also make the surface of the support electrostatically negative, thereby minimizing the association of the negatively-charged DNA tether with the surface. Alternatively, hydrophobic lipid groups may be coupled to the glass surface to discourage DNA-surface association due to the incompatibility of hydrophobic-hydrophilic associations. For example, suitable lipid groups may include phosphatidyl ethanolamine.
In an alternative implementation, the sequences present in adjacent anchor oligonucleotides are synthesized in series (i.e. as a single oligonucleotide). This effectively generates a common anchor for both the first and second tethers and ensures that the swept volumes entirely overlap. There may be advantages to this approach if the binding of very low numbers (as low as 1 pair) of biomolecules were to be studied. In a variant of this implementation, where the first and second biomolecules are not tethered to a separate solid surface, the first and second biomolecules may be tethered at the respective ends of a single tether and measurements could be made in solution.
In a preferred method of connecting protein biomolecules to nucleic acid tethers, protein nucleic acid conjugates are produced according to the method described in: Jung, G. Y., and Stephanopoulos, G. (2004) A functional protein chip for pathway optimization and in vitro metabolic engineering Science 304, 428-431. This description is in turn based on the original method described in: Roberts, R. W., and Szostak, J. W. (1997) RNA-peptide fusions for the in vitro selection of peptides and proteins Proc. Natl. Acad. Sci. U.S.A 94, 12297-12302. In short, the method involves the use of an in vitro translation reaction to covalently attach a nascent peptide by its C-terminus close to the 3′ end of an mRNA-DNA conjugate. An additional class of methods for connecting protein biomolecules to nucleic acid tethers that can be used with equal preference to the method described above. These methods generically involve the synthesis of a fusion protein comprising the biomolecule of interest attached to a modified enzyme (shown schematically in the accompanying
There are three main advantages to the use of the approach described in Jung and Stephanopoulos (2004) supra in the context of the present invention. First, the protein-nucleic acid complex can be purified away from in vitro translation extract proteins, following annealing to the immobilised tethers and washing. Second, multiple messenger RNAs can be simultaneously translated and conjugated to their unique coding nucleic acids; this enables high throughput approaches to be taken to protein production. Third, the proteins produced in the in vitro translation extracts (˜150 ng/translation) are in a large excess over that required to saturate a typical 100 μm diameter microarray spot of tethers (˜8 pg of a 50 KDa protein in a spot containing 30 nm inter-anchor distance with 1×107 molecules). Jung and Stephanoupoulos (2004) showed that the density of ‘oligonucleotide anchors’ in their approach was the primary determinant of the levels of immobilized nucleic acid-protein complexes. In an entirely analogous fashion, the proportion of tethers used in a method in accordance with the invention will determine the proportions of tethered first and second nucleic acid-protein complexes.
Alternative methods of making protein-nucleic acid conjugates may be used, including the direct chemical crosslinking of purified protein biomolecules to modified oligonucleotides. As an alternative, protein-nucleic acid complexes may be generated in situ by annealing the mRNA-DNA conjugate to the immobilized tether first and translating the messenger RNA, whilst bound to the tether, by adding in vitro translation extracts to the tethered messenger RNA.
Alternatively, messenger RNA may be designed to generate protein fusions between the protein biomolecules of interest and a second protein domain X. The second domain X may be designed to have a very high affinity for an engineered component of the head oligonucleotide or the head end of the tether. For example, if the X domain is a high affinity specific DNA binding protein (e.g. lambda repressor), its cognate DNA site may be introduced into the head oligonucleotide complex to enable the nascent protein to associate with the tether via the DNA binding moiety. Alternatively, X could be a molecule such as streptavidin and a corresponding binding partner—in this case biotin—would be chemically coupled to the head oligonucleotide.
Typical protein biomolecules include enzymes, antibodies and receptors. In further alternative methods, the first and/or second biomolecule may be a bioactive molecule other than a protein. The only requirement is that the alternative biomolecule is capable of maintaining its functional activity whilst being coupled to a tether. Alternative molecules include peptides, peptide analogues, such as synthetic amino acids, combinatorial polymer libraries, small molecules (say <1000 Daltons, for example chemically-synthesized drugs), polysaccharides, and catalytically active RNA species.
In a preferred method, nucleic acid protein conjugates are annealed through complimentary sequences, provided by either of the first and second biomolecules, close to the 3′ end of the nucleic acid component to complementary sequences in a head oligonucleotide tether portion. This concentrates the nucleic acid conjugates from molarities typical of in vitro translations (e.g. 10 nM) to the experimental concentrations.
Simple well-characterised equilibrium binding equations (Michaelis Menten) can be used to derive molecular interaction parameters based on the concentrations of the first and second biomolecules and the proportion of first biomolecule/second biomolecule bound.
For example, in a typical experiment to accurately determine the Kd of an interaction between first and second biomolecules which are tethered to a support, first and second biomolecules having a range of tether lengths and inter-anchor distances is set up as an array of spots using appropriate combinations of anchors and tethers for the first and second biomolecules. This generates a standard range of concentrations. These concentrations are first plotted against the proportion of bound first/second biomolecule complex and the concentration of the first biomolecule (or the second biomolecule) required for half maximal binding is determined (this concentration is the Kd).
According to a further aspect of the invention there is therefore provided a method of determining the Kd of an interaction between first and second biomolecules by determining the proportion of bound first and second biomolecules for a range of concentrations of the first and second biomolecules and the determining the concentration of the first or second biomolecule required for half maximal binding of the first and second biomolecules—the Kd. The affinity of a first biomolecule to a library of second biomolecules may be determined. The library of biomolecules may comprise at least a significant portion of a transcriptome or proteome.
Methods in accordance with the invention offer the potential of screening interactions between a single biomolecule A and a library of molecules B1, B2, B3 . . . Bn. In one format, each spot is occupied by only biomolecule A and B1 or A and B2 . . . A and Bn. In a preferred implementation for protein molecules, head tether portions recognising unique (for example coding) regions from the 3′ end of messages B1, B2, B3 . . . Bn are generated and coupled to the core tethers as described earlier. Bn may be libraries of proteins potentially representing a transcriptome/proteome. Alternatively, Bn may be libraries of peptides used for defining interaction sites. Alternatively, Bn may be tethered libraries of chemical compounds ranging from small molecule compounds to libraries of synthetic polymers.
By using an anchor/tether for the second biomolecule that can be cleaved together with initial saturating concentrations of the first and second biomolecules, it is possible to determine Koff. In this scheme, the rate of decay of first biomolecule/second biomolecule complex levels is monitored in real time following cleavage of the tether for the second biomolecule. This type of analysis is analogous to that used in surface plasmon resonance to determine the Koff.
The effect of a third, tethered or non-tethered biomolecule on the interaction between the tethered first and second biomolecules may also be studied.
According to a further aspect of the invention there is provided a method in which the Koff value for an interaction between the first and second biomolecules is determined by providing initial saturating concentrations of the first and second biomolecules, cleaving a second biomolecule tether portion or anchor and monitoring any change in levels of bound first and second biomolecules.
According to a further aspect of the invention there is provided a method of determining the change in free energy (ΔG°) value for an interaction between a first and second biomolecules, the method comprising determining the proportion of bound biomolecules at a first temperature and determining the proportion of bound biomolecules at a second temperature and comparing the proportion of bound biomolecules at the respective first and second temperatures. Typically, the temperature of the biomolecules may be varied by altering the temperature of the experimental apparatus used to perform the method.
According to another aspect of the invention there is provided apparatus for determining the affinity of first and second biomolecules, the apparatus comprising a first biomolecule tethered by a first tether having a first tether length, a second biomolecule tethered by a second tether having a second tether length, means for determining binding of adjacent first and second biomolecules to each other, and means for varying at least one of the first, and second tether lengths.
At least one of the first and second biomolecules may be tethered to a surface of the apparatus. Preferably, both the first and second biomolecules are tethered to a surface. The biomolecules may be tethered separately to the surface or together in, for example, a Y-shaped or linear arrangement. Alternatively, the biomolecules may be tethered together and associated with the apparatus in the form of a solution.
The surface may be provided by a solid support. Preferably, the solid support is a glass slide. Alternatively, the solid support may be a micro bead.
Other aspects of the apparatus may be provided by preferred method features described above.
Methods and apparatus in accordance with the invention will now be described, by way of example, with reference to the further accompanying
-
- A. is an illustration of spheres swept by the free ends of short and long flexible tethers;
- B. is an illustration of a possible conformation of free and bound variants of a linear molecule representing an intra-molecular interaction between biomolecules A and B;
- C. is an illustration of free and bound variants undergoing inter-molecular interactions between A and B;
-
- A. shows separate molecules of the form shown in
FIG. 12C ; - B. shows a linear molecule with acceptor and donor head sets attached.
- A. shows separate molecules of the form shown in
This molecule takes the form shown in
-
- a. a range of lengths; and
- b. a range of concentrations;
The preparation of one form of tethered biomolecules for use in a method in accordance with the invention is shown in
a) Production of Tether Head Portions
Tether body portions are generated from double stranded DNA (dsDNA) as shown particularly in
b) Production of Tether Body Portions
Tether body portions are generated from double stranded DNA (dsDNA) as shown particularly in
c) Production of Tether Tail Portions
Tether tail portions are designed to anneal and ligate to the dsDNA tether body portion and also to anneal to specific anchor oligonucleotides which are described below. The tether tail portions 52 and 54 shown in
d) Assembly of the Tethers
Separate tether production reactions are set up to generate pools of first or second fluorophore or to quantum dot labelled tethers with different tether lengths. The tether head portions 38, 40, tether body portions 50 and tether tail portions 52, 54 are assembled by conventional conditions under suitable conditions in solution as shown in
e) Anchor-Oligonucleotides
The assembled tethers 55, 57 can be anchored to a surface by means of anchors. The anchors are typically single-stranded amino-modified oligonucleotides. In a preferred embodiment, the solid support is a modified glass substrate prepared using standard techniques to covalently couple the anchor oligonucleotide. For example, see: Chrisey, L. A., Lee, G. U., and O'Ferrall, E. (1996) Covalent attachment of synthetic DNA to self-assembled monolayer films Nucleic Acids Res. 24:3031-3039. The amino-modified anchor oligonucleotides are coupled to glass treated with amino silane and p-phenylene1,4 diisothiocyanate (PDC) (
In the specific implementation described below (
As shown in
a) Use of In Vitro Translation
Protein biomolecule/nucleic acid conjugates which can hybridise to the tethers are produced according to the method described in: Jung, G. Y., and Stephanopoulos, G. (2004). supra by an in vitro translation reaction to covalently attach a nascent peptide by its C-terminus close to the 3′ end of an mRNA-DNA conjugate. Tether protein complexes are then hybridised to the annealed arrays of tethers attached to their immobilised anchor oligonucleotides.
This is schematically illustrated in
b) Generation of Protein-Nucleic Acid Complexes In Situ
Alternatively, protein nucleic acid complexes may be generated in situ by annealing the mRNA-DNA conjugate to the immobilized tether first and translating the messenger RNA whilst bound to the tether by adding in vitro translation extracts to the tethered messenger RNA.
c) Use of Protein-Protein Fusions
In another approach, the messenger RNA is engineered to generate protein fusions between the protein biomolecule of interest and a second protein domain X. The domain X is designed to have a very high affinity for an engineered component of a tether head portion oligonucleotide or the head end of the tether. For example, where the X domain is a high affinity specific DNA binding protein (e.g. lambda repressor), its cognate DNA site is introduced into the head oligonucleotide complex to enable the nascent protein to associate with the tether via the DNA binding moiety. Alternatively, X is a molecule such as streptavidin and its binding partner—in this case biotin—is chemically coupled during synthesis to a tether head portion oligonucleotide.
4 ANNEALING OF NUCLEIC ACID—PROTEIN CONJUGATES TO TETHERSIn the preferred method, nucleic acid biomolecule protein conjugates are annealed through complimentary sequences (A or B) close to the 3′ end of the nucleic acid component to complementary sequences in the head tether portion as shown in
As noted above the tethers need not be made from dsDNA but may be made from other molecules such as DNA DX hybrids.
5 MEASUREMENT OF AFFINITY IN SOLUTIONThe measurement of affinity between first and second biomolecules A and B can also be carried out in solution, allowing the basic principle underlying the tethering principle to be investigated using the simplified scheme shown in
In the specific examples described below, Forster Resonance Energy Transfer (FRET) coupled with Fluorescence Life-time Measurement (FLIM) was used to determine the proportion of A and B that were molecularly close in an AB complex. FLIM exploits the time-dependence of FRET to allow more sensitive measurements of the proportions of A and B that are found in AB complexes. Both FRET and FLIM were used in the assays shown. (Backsai et al (2003) J Biomed Opt. 2003 July; 8(3):368-75; Forster T (1965) Delocalized excitation and excitation transfer. In Modern Quantum Chemistry, part III. O. Sinanoslu, editor. Academic Press, New York. 93-137. Stryer L and Haugland R P, (1967) Proceedings of the National Academy of Science USA. 58: 719-730.).
EXAMPLE 1a) Oligonucleotide Labelling and Preparation of ‘Head Sets’
The details of the test system are illustrated in
b) Linear DNA Tether Preparation
To make the longer tethered molecules illustrated in
c) Sample Preparation, FRET and FLIM Detection
Head sets or dual-labelled linear DNA molecules were diluted to the concentrations described in a final concentration of 70 mM NaCl, 10 mM Tris pH 8.0. 6 μl of each solution was introduced into one of the wells of a 50 well slide produced using a multi-chambered coverslip (Stratech Scientific, UK) together with a 22×50 mm coverslip (Menzel-Glaser, Germany).
Samples were analysed using a frequency-doubled Ti:Sa laser providing short optical pulses (100 fs duration) at 76 Mhz repetition rate, with wavelength in the absorption band of the donor fluorophore (˜470 nm). The exciting light was weakly focused onto the sample allowing for a uniform illumination and collection over 1 mm well depth, to maximize the signal contribution over the fluorescence background of the coverslip. Low excitation intensities (0.05-10 mW over 0.4 mm spot diameter) were maintained to avoid nonlinearities and photodamage. Fluorescence light collected from a microscope objective was spectrally analysed using a spectrometer and detected by a cooled CCD camera for time-integrated FRET spectra. For time-resolved FLIM, fluorescence light was filtered by the spectrometer around the emission maximum of the donor fluorophore (520±5 nm) and detected by a single channel fast photomultiplier (200 ps time resolution) connected to a time-correlated single photon counting module. Background contributions were measured from the buffer solution without fluorophores in the same excitation and detection conditions and properly subtracted to the data.
d) Preparation of a Y-Shaped Molecule
The first and second tether portions for each biomolecule in a Y-shaped molecule are anchored to a single DNA strand such that the tethers are free to diffuse as for the linear molecule shown in
e) Data Analysis
To determine the % maximal binding, we first determined the proportion of bound and unbound donor (R) at different donor and acceptor concentrations using the following procedure. The ratio between the bound and unbound decay spectra for different acceptor concentrations was determined over time and plotted as shown in
For each curve a numerical fit (dotted lines) to the decay curve (R(t)=U(1+R exp(−t/τ)) was performed, where R=ratio between bound and unbound donor, t=time, U=N(unbound)/N (where N=concentration of donor in the absence of acceptor). τ=decay constant. R, U and τ were directly determined from the numerical fit of the experimental data.
The proportion of bound donor=R/(1+R) was plotted against acceptor concentration as shown in
f) Theoretical Determination of DNA Binding Affinity
Assuming a chemical reaction between molecules A and D in order to form bound molecule AD:
A+DAD (1)
as well as a reverse reaction and that the system is in equilibrium, we can define dissociation constant:
kd=[A][D]/[AD] (2)
Note that according to the basic textbooks (see for example John SantaLucia, Jr. and Donald Hicks. (2004) Annu. Rev. Biophys. Biomol. Struct. 33, 415-40), people also use equilibrium constant keq=1/kd.
kd=1/keq=exp(ΔG/RT) (3)
where kd [mol/l] is dissociation constant, ΔG [cal/mol] is change of the free energy due to reaction, R=1.987 [cal/(K mol)], T [K] absolute temperature. In order to calculate kd we have to calculate ΔG. In our case we have DNA headsets with different base pairs overlap.
This can be done by methods and software developed by Prof. SantaLucia and co-workers John SantaLucia, Jr. and Donald Hicks. (2004) supra, Annu. Rev. Biophys. Biomol. Struct. 33, 415-40.
In order to estimate properly ΔG for DNA molecules we have to take in account folding and hybridization prediction (M. Zuker. Nucleic Acids Res. 31 (13), 3406-15, (2003)).
The final results are presented in the following tables. The theoretical affinities were calculated using methods described in the following references: John SantaLucia, Jr. and Donald Hicks. (2004) supra; M. Zuker, (2003) supra; and A V Fotin et al, Nucleic Acids Res. 26 (1998) p. 1515.
The results presented in Tables 3 and Table 4 for 11 base pairs with a correction due to the folding depend on the methods for the calculation which is used either SantaLucia or Fotin. The difference is one order of magnitude. For 9 base pairs the agreement between two methods is better.
Resultsa) Determination of the Binding Affinity of the 11 bp Overlap using Free Oligonucleotides
An essential initial goal of these studies was to determine an accurate value for the 11 bp affinity to enable later comparison with results using the nano-tether methodology of the invention. Standard titration reactions were carried out to identify the dissociation constant (Kd) for the oligonucleotides shown in
To determine the amount of D:A hybrids, the samples were analysed for the time-dependence of FRET-FLIM as described above. A representative plot from this analysis is shown in
The characteristic decay curves from FRET-FLIM analyses of the kind shown in
b) Tether Length-Dependence of FLIM on Linear Molecules
The proportion of linear tether molecules found in the bound form increased as the length of the tether decreased according to predictions (
The percentage maximal FLIM was plotted against nominal tethered concentration in
The generation of the data shown involved the preparation of fluorophore-labelled linear DNA molecules and the measurement of time resolved FRET.
1 Preparation of Reagents a) Design of the Head SetsThe biomolecules whose affinity was measured are shown in
The overlapping oligonucleotide pairs are called ‘Head Sets’ and they are distinguished by the attached fluorophore. The donor fluorophore (Alexafluor 488) and Acceptor (ATTO550) fluorophores were attached to the oligonucleotides during synthesis by commercial suppliers (Eurogentec) and are attached to bases indicated.
As a control, analogous fluorophore-labelled Head Set blunt-ended oligonucleotides were synthesised that have no single stranded overlap (0 bp overlap;
The 2 constituent oligonucleotides for the donor or acceptor Head Sets (25 μM final concentration) were annealed by cooling from 90° C. to room temperature over 1 hour in a thermal cycler machine in annealing buffer (70 mM NaCl 10 mM Tris pH 7.4).
Following annealing, 1.5 μl of a 25 μM solution of each of the donor and acceptor Heat Sets (˜5 fold molar excess) was ligated to various length ‘Tether Body’ DNAs to generate linear molecules with a terminal donor and acceptor Head Set according to standard procedures ((Sambrook et al., 1989);
The DNAs that were analysed by FRET (
Following ligation, the linear molecules were gel purified and quantified by comparison with known DNA standards. For FRET analysis, the samples were diluted to the concentrations indicated and 5 μl was added to the wells of a multiwell chambered coverslip (Grace Bio-labs; CWCS 50R-1.0). The wells were sealed with a standard glass coverslip.
2 Time-Resolved FRET Analysis. a) Data AcquisitionSamples were analysed using a frequency-doubled Ti:Sa laser providing short optical pulses (100 fs duration) at 76 Mhz repetition rate, with wavelength in the absorption band of the donor fluorophore (˜470 nm). The exciting light was weakly focused onto the sample allowing for a uniform illumination and collection over 1 mm well depth, to maximize the signal contribution over the fluorescence background of the coverslip. Low excitation intensities (0.05-10 mW over 0.4 mm spot diameter) were maintained to avoid nonlinearities and photodamage. Fluorescent light collected from a microscope objective was spectrally analysed using a spectrometer and detected by a cooled CCD camera for time-integrated FRET spectra. For time-resolved FRET, fluorescence light was filtered by the spectrometer around the emission maximum of the donor fluorophore (520±5 nm) and detected by a single channel fast photomultiplier (200 ps time resolution) connected to a time-correlated single photon counting module. Background contributions were measured from the buffer solution without fluorophores in the same excitation and detection conditions and properly subtracted to the data.
b) Data AnalysisThe time dependence of FRET can be seen in the Donor and Acceptor dynamics shown in
The proportion of bound (circular conformation) to total number of molecules [Dbound/Dtot] is proportional to the probability that the molecules are in the circular conformation and was calculated as described above.
The variation of the proportion of bound molecules with the length of DNA is shown in
The second major point to note is that the proportion of bound molecules was not markedly affected by a 10 fold dilution (10 nM to 1 nM;
The results show that tethered biomolecules at each end of a linear DNA tether occupy an effective volume that is close to that predicted on the basis of the swept volume of their contour length, d (4/3.pi.(d/2)3). The data shows that varying the length of the tether alters the effective concentration of the ends.
These results show that tether length can be used as a direct way of controlling the concentration of biomolecules at the free ends of the tethers and that a high ‘concentration’ of tethered biomolecules can be obtained via an intra-molecular interaction between a pair of biomolecules at the end of the tether.
The results show that FRET/FLIM analysis is a practical way of assessing the proportion of bound biomolecules attached at the end of the tethers. As the percentage of interacting molecules is dependent on the length of the tether and not on the concentration of the tethers, it is, in principle, possible to measure the affinity of a pair of tethered molecules by taking multiple FRET/FLIM readings on a single tethered molecule. However, with the sensitivity of existing fluorescence technologies, we estimate that FRET/FLIM analyses will require at least 10,000 tethered molecule pairs necessary to estimate an equilibrium binding constant since readings will need to be made with as few as 10% of bound pairs 1,000 molecules. Nonetheless, this number of molecules is in the attomole range and argues that the technique should be as sensitive as discussed above.
Although the preferred method for tethering the biomolecules is to attach them to a solid surface, the connection of two biomolecules via a single flexible tether is essentially a minor practical modification of the linear tether system described since the primary control over tethered biomolecule concentration will be attained by altering the tether length. However, the surface tethered method should also allow fine control of the overlap between swept volumes by altering the inter-anchor distances (see
Nonetheless, we note that the linear molecule and other implementations of the nano-tether biochemistry approach such as the Y-shaped molecule (
a) Glass Slide Format
In one embodiment, the format of the support is a glass slide onto which oligonucleotides have been printed in arrays of spots using a split pin arraying machine.
b) Microbead Format
In an alternative format, the support is provided by microbeads that are coupled in formats that generate a unique relationship between a single bead and tether combination. This format enables the adaptation of the technology to microfluidic systems.
c) Controlling the Inter-Anchor Spacing
Using the preferred arrayed-spot implementation, mentioned in section 6a) above, amino-terminal oligonucleotide anchors for the first and second biomolecules are covalently coupled to the modified glass substrate. A non-specific amino-terminal oligonucleotide (designed not to bind tether components) is titrated into the anchor oligonucleotide coupling mix to vary the inter-anchor coupling distance where appropriate. Inter-anchor mean distances are varied from lengths greater than the tether length to the maximal oligonucleotide tether capacity (maximal capacity is 20 pmoles of bound DNA/cm2 which equates to an mean inter-anchor spacing of 1.6 nm; Chrisey, L. A., et al (1996)). This inter-anchor density massively exceeds that required for the typical range of anchor densities (e.g. to bring 200 bp (60 nm) tethers within a mean 30 nm of each other requires a mean spacing of 30 nm).
The non-specific oligonucleotide functions to cap the reactive groups and will also make the surface electrostatically negative, thereby minimizing the association of the negatively-charged DNA tether with the surface. Alternatively, hydrophobic lipid groups may be coupled to the glass surface to discourage DNA-surface association due to the incompatibility of hydrophobic-hydrophilic associations.
In an alternative implementation, the sequences present in the anchor oligonucleotide (sequences 1 and 2; of anchors 56 and 58 in
a) Slide Mounted Systems
In one embodiment of the invention, the assay readout is the intensity of Forster resonance energy transfer (FRET) between the different fluorophores 42, 43 coupled to the tether head portions 38 and 40 or elsewhere in the nucleic acid portion of the tether as shown in
FRET is measured using a confocal microscope on glass slides containing arrays of tethered biomolecules.
b) Use of Nanoscale Spheres or Quantum Dots
In an alternative solution, nanoscale solids, such as spheres or “quantum dots” (Doty, R. C. et al Cell Mol. Life Sci. 61 (15) 1843-9), are tethered in place of the single fluorophores. These conjugates may offer higher FRET efficiencies due to the increased number of fluorescent molecules. Alternatively, the nanoscale solids would allow fluorescence correlation spectroscopy to be performed using a high-resolution light confocal microscope. For tethers longer than 2 Kb (0.6 μm), the formation of first and second biomolecule complexes can be directly recorded due to the proportion of fluorescent dots pairs in proportion to those that show some separation.
8 DATA ANALYSISSimple well characterised equilibrium binding equations (Michaelis Menten) are used to derive molecular interaction parameters based on the concentrations of the first and second biomolecules and the proportion of those biomolecules which are bound.
9 APPLICATIONSAdditional applications of, methods of the present invention, the nano-tether biochemistry technique, in all formats (linear, Y-shaped and attached) include:
a) Determination of Kd
For example, in a typical experiment to accurately determine the Kd of an interaction, a range of tether lengths and inter-anchor distances are set up as an array of spots using appropriate combinations of anchors and tethers for the first and second biomolecules. This generates a standard range of concentrations. These concentrations are plotted against the proportion of bound first and second biomolecule complex and the concentration of the first biomolecule (or the second biomolecule) required for half maximal binding is determined (This concentration is the Kd).
b) Library Screening
The method of invention allows the screening of interactions between a single molecule A and a library of molecules B1, B2, B3 . . . Bn. In this format, each spot is occupied by only A and B1 or A and B2 . . . A and Bn. In a preferred implementation for protein molecules, head tethers recognising unique (for example coding) regions from the 3′ end of messages B1, B2, B3 . . . Bn are generated and coupled to the core tethers as described earlier. Bn can be a library of proteins potentially representing the transcriptome/proteome. Alternatively, Bn can be libraries of peptides used to defining interaction sites or tethered libraries of chemical compounds ranging from small molecule compounds to libraries of synthetic polymers.
c) Koff Measurement
As illustrated schematically in
This may be achieved in two ways. For situations involving slow Koff rates, restriction enzyme digestion of the anchor/tether releases the second biomolecule and allows it to diffuse away from the first biomolecule. For faster Koff rates, a modified oligonucleotide containing a photo-cleavable moiety is incorporated into the single stranded region of the anchor. The photocleavage is initiated using a different wavelength of light from that used in FRET analysis. By knowing Koff and Kd, Kon, can be calculated based on the equation Kd=Koff/Kon
d) Screening for Modulators of Biological Systems
By establishing binding constants between the first and second biomolecules that are close to the Kd, it is possible to set up binding reactions at concentrations of the first and second biomolecules that are close to the Kd and thus are particularly sensitive to screens for soluble modulators of their interaction. These modulating molecules will collectively be called “C”. Examples of C include: a purified interacting protein, a protein that modifies A and B (e.g. a kinase), a drug molecule or candidate, complex mixtures of proteins that contain one or more components that alter AB complex formation (e.g. cell extracts, blood serum, other biological fluids). C could be a solution of a single molecule or complex mixtures of compounds (e.g. biological extracts or bodily fluids). C may itself be tethered to a third tether or alternatively it may be non-tethered, for example, in solution according to the application. The presence of C can be tested in a number of formats as described below with reference to
Format 1. An array of different first and second tethered biomolecule pairs is treated with C to determine the range of binding reactions that C affects. The tether lengths of A and B can be adjusted such that their effective concentration would be close to the Kd of the AB complex. At this concentration, 50% of AB would be present in the complex and the interaction would be most sensitive to factors that alter the strength of AB interaction. Factor ‘C’ may increase or decrease the affinity of A for B by interacting with or modifying either or both of A and B.
Format 2. The same tethered pair of first and second biomolecules is treated with different C compounds by tethering the first and second in separate reaction wells (e.g. microwell plates).
Format 3. Continuous Flow. The same tethered pair of first and second biomolecules arranged in a column format or an array of microbeads or in a microfluidic system will be treated in a flow of C. In this case, C may be a sequential series of test solutions or fractions from a separation (e.g. Chromatography column eluates in a combinatorial chemistry system, or protein fractions from a cellular extract).
Format 4. Measurement of concentration of known ‘C’s. When the affinity of a Factor ‘C’ for A, B or an AB complex is known, the concentration of Factor C can be measured. This could be used for example to determine the proportion of biomolecules in clinical samples such as serum.
Claims
1-74. (canceled)
75. An assembly comprising a plurality of tethered biomolecules, each member of said plurality comprising
- a first biomolecule tethered by a first tether portion having a first tether portion length and a first tether persistence length and
- a second biomolecule tethered by a second tether portion having a second tether portion length and a second tether persistence length,
- wherein the first and second biomolecules are tethered together such that a swept volume is defined for each member of said plurality by the first and second tether portion lengths,
- and members of said plurality also having means for determining binding of first and second biomolecules to each other.
76. The assembly of claim 75, wherein the first and second tether portions are provided by a single tether.
77. The assembly of claim 75, wherein at least one member of said plurality is in solution.
78. A method of measuring the affinity of a first and a second biomolecule comprising
- providing a plurality of tethered biomolecules in solution,
- each member of said plurality comprising
- a first biomolecule tethered by a first tether portion having a first tether portion length and a first tether persistence length and
- a second biomolecule tethered by a second tether portion having a second tether portion length and a second tether persistence length, wherein the first and second biomolecules are tethered together such that a swept volume is defined for each member of said plurality by the first and second tether portion lengths,
- and members of said plurality also having means for determining binding of first and second biomolecules to each other;
- varying at least one of said first and/or second portion lengths and/or said first and/second persistence lengths; and
- measuring the binding of the first and second biomolecules.
79. The method of claim 78, wherein a range of the first and second tether portion lengths produce a range of effective concentrations for the first and/or second biomolecules.
80. The method of claim 79, wherein said method further comprises determining the binding of the first and second biomolecules in the presence of a third biomolecule.
81. The method of claim 79, wherein the length of the first and/or second tether portion are different.
82. The method of claim 78, wherein the at least one tether portion comprises nucleotides.
83. The method of claim 78, wherein the at least one tether portion comprises a double-stranded DNA.
84. The method of claim 78, wherein the at least one tether portion comprises a carbon nanotube, an amyloid fibril, or a polymer.
85. The method of claim 84, wherein the polymer is a DNA crossover complex.
86. The method of claim 78, wherein said first and/or second tether portions are made from double-stranded DNA, DX hybrids, carbon nanotubes, amyloid fibrils, or polymers to produce a range of effective concentrations for the first and/or second biomolecules.
87. The method of claim 78, wherein the proportion of the first and second biomolecules that are molecularly close to each other indicates the proportion of interacting the first and second biomolecules.
88. The method of claim 78, wherein the proportion of binding of the first and second biomolecules is determined by the intensity of fluorescence (Forster) resonance energy transfer (FRET) between a first and second fluorophores respectively attached to, or integrated with, the first and second biomolecules.
89. The method of claim 78, wherein the Kd of an interaction between the first and second biomolecules is determined by determining the proportion of the first and second biomolecules bound to each other for a range of concentrations of the first and second biomolecules and determining the concentration of the first or second biomolecule required for half maximal binding of the first and second biomolecules.
90. The method of claim 78, wherein the Koff value for an interaction between the first and second biomolecules is determined by providing initial saturating concentrations of the first and second biomolecules, cleaving the second tether portion and monitoring any change in levels of bound first and second biomolecules.
91. The method of claim 78, wherein said method further comprises providing a concentration of the first and second biomolecules around the Kd of an interaction between the first and second biomolecules and determining the effect of a modulator on the portion of the first and the second biomolecules bound to each other.
92. The method of claim 78, wherein the second biomolecule is selected from a library.
93. The method of claim 78, wherein the method further comprises changing said first and/or second persistence length of said first and/or second tethers of the first and/or second tether portion by chemical modification or physical association of the first and/or second tether portion to produce a range of effective concentrations for the first and/or second biomolecules.
94. A method of measuring the affinity of a first and a second biomolecule, wherein the first biomolecule is tethered by a first tether portion having a first tether portion length and a first tether persistence length and the second biomolecule is tethered by a second tether portion having a second tether portion length and a second tether persistence length, wherein the first and second biomolecules are tethered to a surface, such that swept volumes defined by the movement of each biomolecule overlap, so that the first and second biomolecules are able to bind to each other, said method comprising determining a proportion of the first and second biomolecules bound to each other.
Type: Application
Filed: Jul 7, 2017
Publication Date: Dec 28, 2017
Inventors: Trevor Clive DALE (Cardiff), Adrian John HARWOOD (Cardiff), Paola BORRI (Cardiff)
Application Number: 15/644,078