Rapid mixing kinetic techniques.

Methods Mol Biol

Division of Physical Biochemistry, MRC National Institute for Medical Research, London, UK.

Published: December 2013

AI Article Synopsis

  • Many biochemical reactions occur quickly, often in less than a second, so traditional methods of mixing and monitoring concentrations aren't effective for studying these fast processes.
  • Rapid mixing techniques that mix reagents in under 2 milliseconds allow for the study of reactions that reach equilibrium, with specific applications in enzyme kinetics mentioned in various textbooks.
  • Common monitoring methods for reactions include observing changes in optical signals like absorbance or fluorescence, though fluorescence is often favored for its sensitivity; however, for precise concentration measurements, discontinuous methods like HPLC can be used, albeit with lower time resolution.

Article Abstract

Almost all of the elementary steps in a biochemical reaction scheme are either unimolecular or bimolecular processes that frequently occur on sub-second, often sub-millisecond, time scales. The traditional approach in kinetic studies is to mix two or more reagents and monitor the changes in concentrations with time. Conventional spectrophotometers cannot generally be used to study reactions that are complete within less than about 20 s, as it takes that amount of time to manually mix the reagents and activate the instrument. Rapid mixing techniques, which generally achieve mixing in less than 2 ms, overcome this limitation. This chapter is concerned with the use of these techniques in the study of reactions which reach equilibrium; the application of these methods to the study of enzyme kinetics is described in several excellent texts (Cornish-Bowden, Fundamentals of enzyme kinetics. Portland Press, 1995; Gutfreund, Kinetics for the life sciences. Receptors, transmitters and catalysis. Cambridge University Press, 1995).There are various ways to monitor changes in concentration of reactants, intermediates and products after mixing, but the most common way is to use changes in optical signals (absorbance or fluorescence) which often accompany reactions. Although absorbance can sometimes be used, fluorescence is often preferred because of its greater sensitivity, particularly in monitoring conformational changes. Such methods are continuous with good time resolution but they seldom permit the direct determination of the concentrations of individual species. Alternatively, samples may be taken from the reaction volume, mixed with a chemical quenching agent to stop the reaction, and their contents assessed by techniques such as HPLC. These methods can directly determine the concentrations of different species, but are discontinuous and have a limited time resolution.

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http://dx.doi.org/10.1007/978-1-62703-398-5_5DOI Listing

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