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Figure 1. A fraction of receptor not bound to ligand in solution is captured by the ligand coated solid phase and subsequently labelled with a fluorescent secondary antibody.

A kinetic exclusion assay (KinExA) is a type of bioassay in which a solution containing receptor, ligand, and receptor-ligand complex is briefly exposed to additional ligand immobilized on a solid phase.[1][2]

Description[edit]

During the assay, a fraction of the free receptor is captured by the solid phase ligand and subsequently labeled with a fluorescent secondary molecule (Figure 1).[1][2] The short contact time with the solid phase does not allow significant dissociation of the pre-formed complexes in the solution.[3] Solution dissociation is thus “kinetically excluded” from contributing to the captured receptor and the resulting signal provides a measure of the free receptor in the solution.

Measuring the free receptor as a function of total ligand in a series of equilibrated solutions enables calculation of the equilibrium dissociation constant (Kd).[1][2][3][4][5][6][7][8] Measuring the free receptor with several points before equilibrium enables measurement of the association rate constant (kon). The off rate (koff) can also be directly measured, however it is usually calculated from the measured Kd and measured kon, (koff = Kd * kon).

Kinetic exclusion assays have been used to measure Kd’s in the nanomolar to femtomolar range.[4][5][6][7][9][10]

Applications[edit]

Figure 2. Example of signal generation. 1) Beads Load. 2) Equilibrated solution passes over column. 3) Introduction of secondary label. 4) Fluorescent emission of captured free receptor.

Because the fluorescent secondary molecule is applied after capture of the free receptor from solution (Figure 2) the binding constants measured using a kinetic exclusion assay are for unmodified molecules in solution and thus more accurately reflects endogenous binding interactions than methods requiring modification (typically labeling or immobilization) before measurement.[1][2] Kinetic exclusion assays have been performed using unpurified molecules,[4][5] in serum,[7] and have measured binding to cell membrane proteins on intact whole cell[8][11] which brings the measured binding interactions closer to their endogenous state.

Molecules suited for measurement by KinExA are antibodies,[4][7][12][13][14] recombinant proteins,[15][16][17] small molecules,[6][18][19][20] aptamers,[21][22] lipids,[23][24] nanobodies,[25] and toxins.[12][26][27]

Kinetic exclusion assay have also been applied for concentration immunoassay, where it has proven capable of providing the maximum theoretical, Kd limited, sensitivity.[28][29] An example of this technique has been employed for sensitive detection of environmental contaminants in near real-time.[30]

Standard equilibrium affinity analysis[edit]

A series of samples are prepared with all the same receptor (R) concentration but in which the ligand (L) concentration is titrated. After equilibrium is reached each sample is measured by flowing it through the column (Figure 2).

For 1:1 reversible binding Equilibrium Kd is defined as

(1) Kd≡koff/kon =R*L/RL

the binding is reversible so conservation of mass can be written as

(2) RT = R+RL

(3) LT = L +RL

Where:

Kd = equilibrium dissociation constant

kon = forward rate constant

koff = reverse rate constant

R = free receptor site concentration at equilibrium

L = free ligand site concentration at equilibrium

RL = concentration of complex at equilibrium

RT= total concentration of receptors

LT = total concentration of ligand

A simple equation[1][2] relating the free fraction of R (=R/RT) to the Kd and LT is then fit to the measured data to find the Kd of the interaction.

Rate constant analysis[edit]

To measure the rate constants, known concentrations of receptor and ligand are mixed in solution and the quantity of free receptor is repeatedly measured over time as the solution phase reaction occurs. The time course of the free receptor depletion is then fit with a standard bimolecular rate equation.

(4) dLR/dt = kon∙R∙L - Kd∙kon∙RL

where Kd * kon has been substituted for koff .

References[edit]

  1. ^ a b c d e Blake, Robert C.; Pavlov, Andrey R.; Blake, Diane A. (1999). "Automated Kinetic Exclusion Assays to Quantify Protein Binding Interactions in Homogeneous Solution". Analytical Biochemistry. 272 (2): 123–134. doi:10.1006/abio.1999.4176. PMID 10415080.
  2. ^ a b c d e Darling, Ryan J.; Brault, Pierre-Alexandre (2004). "Kinetic Exclusion Assay Technology: Characterization of Molecular Interactions". ASSAY and Drug Development Technologies. 2 (6): 647–657. doi:10.1089/adt.2004.2.647. ISSN 1540-658X. PMID 15674023.
  3. ^ a b Glass, Thomas R.; Winzor, Donald J. (2014). "Confirmation of the validity of the current characterization of immunochemical reactions by kinetic exclusion assay". Analytical Biochemistry. 456: 38–42. doi:10.1016/j.ab.2014.04.011. PMID 24751468.
  4. ^ a b c d Bee, Christine; Abdiche, Yasmina N.; Stone, Donna M.; Collier, Sierra; Lindquist, Kevin C.; Pinkerton, Alanna C.; Pons, Jaume; Rajpal, Arvind (2012-04-30). "Exploring the Dynamic Range of the Kinetic Exclusion Assay in Characterizing Antigen-Antibody Interactions". PLOS ONE. 7 (4): e36261. Bibcode:2012PLoSO...736261B. doi:10.1371/journal.pone.0036261. ISSN 1932-6203. PMC 3340344. PMID 22558410.
  5. ^ a b c Rathanaswami, Palaniswami; Richmond, Karen; Manchulenko, Kathy; Foltz, Ian N. (2011-07-01). "Kinetic analysis of unpurified native antigens available in very low quantities and concentrations". Analytical Biochemistry. 414 (1): 7–13. doi:10.1016/j.ab.2011.02.034. ISSN 1096-0309. PMID 21371417.
  6. ^ a b c Luginbühl, Béatrice; Kanyo, Zoltan; Jones, R. Mark; Fletterick, Robert J.; Prusiner, Stanley B.; Cohen, Fred E.; Williamson, R. Anthony; Burton, Dennis R.; Plückthun, Andreas (2006-10-13). "Directed evolution of an anti-prion protein scFv fragment to an affinity of 1 pM and its structural interpretation". Journal of Molecular Biology. 363 (1): 75–97. doi:10.1016/j.jmb.2006.07.027. ISSN 0022-2836. PMID 16962610.
  7. ^ a b c d Bee, Christine; Abdiche, Yasmina N.; Pons, Jaume; Rajpal, Arvind (2013-11-06). Kaveri, Srinivas (ed.). "Determining the Binding Affinity of Therapeutic Monoclonal Antibodies towards Their Native Unpurified Antigens in Human Serum". PLOS ONE. 8 (11): e80501. Bibcode:2013PLoSO...880501B. doi:10.1371/journal.pone.0080501. ISSN 1932-6203. PMC 3819287. PMID 24223227.
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  12. ^ a b Fan, Yongfeng; Barash, Jason R.; Lou, Jianlong; Conrad, Fraser; Marks, James D.; Arnon, Stephen S. (2016-03-01). "Immunological Characterization and Neutralizing Ability of Monoclonal Antibodies Directed Against Botulinum Neurotoxin Type H". Journal of Infectious Diseases. 213 (10): 1606–1614. doi:10.1093/infdis/jiv770. ISSN 0022-1899. PMC 4837907. PMID 26936913.
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  15. ^ Kariolis, Mihalis S.; Miao, Yu Rebecca; Jones, Douglas S.; Kapur, Shiven; Mathews, Irimpan I.; Giaccia, Amato J.; Cochran, Jennifer R. (2014). "An engineered Axl 'decoy receptor' effectively silences the Gas6/Axl signaling axis". Nature Chemical Biology. 10 (11): 977–983. doi:10.1038/nchembio.1636. ISSN 1552-4450. PMC 4372605. PMID 25242553.
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  17. ^ Champagne, Kelly; Shishido, Akira; Root, Michael J. (2009-02-06). "Interactions of HIV-1 inhibitory peptide T20 with the gp41 N-HR coiled coil". The Journal of Biological Chemistry. 284 (6): 3619–3627. doi:10.1074/jbc.M809269200. ISSN 0021-9258. PMC 2635040. PMID 19073602.
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  19. ^ Chiu, Y. W.; Li, Q. X.; Karu, A. E. (2001-11-15). "Selective binding of polychlorinated biphenyl congeners by a monoclonal antibody: analysis by kinetic exclusion fluorescence immunoassay". Analytical Chemistry. 73 (22): 5477–5484. doi:10.1021/ac0102462. ISSN 0003-2700. PMID 11816577.
  20. ^ Blake, Diane A.; Chakrabarti, Pampa; Khosraviani, Mehraban; Hatcher, Frank M.; Westhoff, Connie M.; Goebel, Peter; Wylie, Dwane E.; Blake, Robert C. (1996-11-01). "Metal Binding Properties of a Monoclonal Antibody Directed toward Metal-Chelate Complexes". Journal of Biological Chemistry. 271 (44): 27677–27685. doi:10.1074/jbc.271.44.27677. ISSN 0021-9258. PMID 8910359. S2CID 35192838.
  21. ^ Leung, Elizabeth; Rohn, Troy; Fologea, Daniel (2018). "Quantifying Protein-DNA Interactions by Kinetics Exclusion Assay". Biophysical Journal. 114 (3): 442a. Bibcode:2018BpJ...114..442L. doi:10.1016/j.bpj.2017.11.2445.
  22. ^ European Patent Office. "EP 2770058 A1 20140827 - Ligand and method for detection of okadaic acid". data.epo.org. Retrieved 2020-07-16.
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  30. ^ Li, Xin; Kaattari, Stephen L.; Vogelbein, Mary A.; Vadas, George G.; Unger, Michael A. (2016). "A highly sensitive monoclonal antibody based biosensor for quantifying 3–5 ring polycyclic aromatic hydrocarbons (PAHs) in aqueous environmental samples". Sensing and Bio-Sensing Research. 7: 115–120. doi:10.1016/j.sbsr.2016.02.003. PMC 4767017. PMID 26925369.
source: https://en.wikipedia.org/wiki/Kinetic_exclusion_assay

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