FUNDAMENTALS OF BIOCHEMISTRY - LL FD
FUNDAMENTALS OF BIOCHEMISTRY - LL FD
5th Edition
ISBN: 9781119598022
Author: Voet
Publisher: WILEY
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Chapter 12, Problem 12E
Summary Introduction

To explain: The reason why the given sets of Lineweaver-Burk plots are not individually ideal for determining KM for an enzyme-catalyzed reaction that follows Michaeli-Menten kinetics.

Concept introduction:

Enzymes are biological protein catalysts which alter the speed of the reaction in the biological system. The chemical reactions which are catalyzed by these enzymes are studied under the enzyme kinetics. The reaction rate is measured based on the rate at which the substrate of the enzymes combines with the enzyme and forms the products. KM is the Michaelis-Menton constant. KM value is not a direct measure of the affinity of the enzyme towards the substrate but concentration of S where the velocity at maximum is half. Vmax is the maximum velocity with which the enzyme catalyzes the reaction.

The rate of enzyme reaction (V) =Vmax[S](KM+[S])

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Problem 15 of 15 Submit Using the following reaction data points, construct Lineweaver-Burk plots for an enzyme with and without an inhibitor by dragging the points to their relevant coordinates on the graph and drawing a line of best fit. Using the information from this plot, determine the type of inhibitor present. 1 mM-1 1 s mM -1 [S]' V' with 10 μg per 20 54 10 36 20 5 27 2.5 23 1.25 20 Answer: |||
12:33 CO Problem 4 of 15 4G 54% Done On the following Lineweaver-Burk -1 plot, identify the by dragging the Km point to the appropriate value. 1/V 40 35- 30- 25 20 15 10- T Км -15 10 -5 0 5 ||| 10 15 №20 25 25 30 1/[S] Г powered by desmos

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FUNDAMENTALS OF BIOCHEMISTRY - LL FD

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Enzyme Kinetics; Author: MIT OpenCourseWare;https://www.youtube.com/watch?v=FXWZr3mscUo;License: Standard Youtube License