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In enzyme kinetics, a secondary plot uses the intercept or slope from several Lineweaver-Burk plots to find additional kinetic constants.

For example, when a set of v by [S] curves from an enzyme with a ping–pong mechanism (varying substrate A, fixed substrate B) are plotted in a Lineweaver–Burk plot, a set of parallel lines will be produced.

The following Michaelis–Menten equation relates the initial reaction rate v₀ to the substrate concentrations [A] and [B]:

{\begin{aligned}{\frac {1}{v_{0}}}&={\frac {K_{M}^{A}}{v_{\max }{[}A{]}}}+{\frac {K_{M}^{B}}{v_{\max }{[}B{]}}}+{\frac {1}{v_{\max }}}\end{aligned}}

The y-intercept of this equation is equal to the following:

{\begin{aligned}{\mbox{y-intercept}}={\frac {K_{M}^{B}}{v_{\max }{[}B{]}}}+{\frac {1}{v_{\max }}}\end{aligned}}

The y-intercept is determined at several different fixed concentrations of substrate B (and varying substrate A). The y-intercept values are then plotted versus 1/[B] to determine the Michaelis constant for substrate B, $K_{M}^{B}$ , as shown in the Figure to the right. The slope is equal to $K_{M}^{B}$ divided by $v_{\max }$ and the intercept is equal to 1 over $v_{\max }$ .

File:Secondary Plot.jpg

Secondary Plot of enzyme system Horseradish Peroxidase and o-Phenylenediamine (with hydrogen peroxide as the second substrate)

Secondary Plot in Inhibition Studies

A secondary plot may also be used to find a specific inhbition constant, k_I.

For a competitive enzyme inhibitor, the apparent Michaelis constant is equal to the following:

{\begin{aligned}{\mbox{apparent }}K_{m}=K_{m}\times \left(1+{\frac {[I]}{K_{I}}}\right)\end{aligned}}

The slope of the Lineweaver-Burk plot is therefore equal to:

{\begin{aligned}{\mbox{slope}}={\frac {K_{m}}{v_{\max }}}\times \left(1+{\frac {[I]}{K_{I}}}\right)\end{aligned}}

If one creates a secondary plot consisting of the slope values from several Lineweaver-Burk plots of varying inhibitor concentration [I], the competitive inhbition constant may be found. The slope of the secondary plot divided by the intercept is equal to 1/k_I. This method allows one to find the k_I constant, even when the Michaelis constant and v_max values are not known.

References

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Template:Refbegin

A. Cornish-Bowden. Fundamentals of Enzyme kinetics, Rev. ed., Portland: London, England, (1995) pp. 30-37, 56-57.
The Horseradish Peroxidase/ o-Phenylenediamine (HRP/OPD) System Exhibits a Two-Step Mechanism. M. K. Tiama and T. M. Hamilton, Journal of Undergraduate Chemistry Research, 4, 1 (2005).
J. N. Rodriguez-Lopez, M. A. Gilabert, J. Tudela, R. N. F. Thorneley, and F. Garcia-Canovas. Biochemistry, 2000, 39, 13201-13209.

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+In [[enzyme kinetics]], a '''secondary plot''' uses the intercept or slope from several Lineweaver-Burk plots to find additional kinetic constants.
+For example, when a set of v by [S] curves from an [[enzyme]] with a ping–pong mechanism (varying substrate A, fixed substrate B) are plotted in a [[Lineweaver–Burk plot]], a set of parallel lines will be produced.
+The following [[Michaelis-Menten kinetics|Michaelis–Menten equation]] relates the initial reaction rate ''v''<sub>0</sub> to the [[substrate (biochemistry)|substrate]] concentrations [A] and [B]:
+:<math>
+\begin{align}
+\frac{1}{v_0} &= \frac{ K_M^A}{v_\max {[}A{]}}+\frac{ K_M^B}{v_\max {[}B{]}}+\frac{1}{v_\max}
+\end{align}
+</math>
+The y-intercept of this equation is equal to the following:
+:<math>
+\begin{align}
+\mbox{y-intercept} = \frac{ K_M^B}{v_\max {[}B{]}}+\frac{1}{v_\max}
+\end{align}
+</math>
+The y-intercept is determined at several different fixed concentrations of substrate B (and varying substrate A).  The y-intercept values are then plotted versus 1/[B] to determine the Michaelis constant for substrate B, <math>K_M^B</math>, as shown in the Figure to the right.  The slope is equal to <math>K_M^B</math> divided by <math>v_\max</math> and the intercept is equal to 1 over <math>v_\max</math>.
+[[Image:Secondary Plot.jpg|thumb|right|300px|Secondary Plot of enzyme system Horseradish Peroxidase and ''o''-Phenylenediamine (with hydrogen peroxide as the second substrate)]]
+==Secondary Plot in Inhibition Studies==
+A secondary plot may also be used to find a specific inhbition constant, k<sub>I</sub>.
+For a competitive [[enzyme inhibitor]], the apparent Michaelis constant is equal to the following:
+:<math>
+\begin{align}
+\mbox{apparent } K_m=K_m\times \left(1+\frac{[I]}{K_I}\right)
+\end{align}
+</math>
+The slope of the Lineweaver-Burk plot is therefore equal to:
+:<math>
+\begin{align}
+\mbox{slope} =\frac{K_m}{v_\max}\times \left(1+\frac{[I]}{K_I}\right)
+\end{align}
+</math>
+If one creates a secondary plot consisting of the slope values from several Lineweaver-Burk plots of varying inhibitor concentration [I], the competitive inhbition constant may be found.  The slope of the secondary plot divided by the intercept is equal to 1/k<sub>I</sub>.  This method allows one to find the k<sub>I</sub> constant, even when the Michaelis constant and v<sub>max</sub> values are not known.
+== References ==
+{{reflist}}
+{{refbegin}}
+* A. Cornish-Bowden. <u>Fundamentals of Enzyme kinetics</u>, Rev. ed., Portland: London, England, (1995) pp. 30-37, 56-57.
+* The Horseradish Peroxidase/ o-Phenylenediamine (HRP/OPD) System Exhibits a Two-Step Mechanism. M. K. Tiama and T. M. Hamilton, ''Journal of Undergraduate Chemistry Research'', '''4''', 1 (2005).
+* J. N. Rodriguez-Lopez, M. A. Gilabert, J. Tudela, R. N. F. Thorneley, and F. Garcia-Canovas. ''Biochemistry'', 2000, '''39''', 13201-13209.
+[[Category:Enzyme kinetics]]

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Secondary Plot in Inhibition Studies

References

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