2-氯-(ε-氨基-Lys75)-[6-[4-(N,N-二乙氨基)苯基]-1,3,5-三嗪-4-基]钙调蛋白与平滑肌肌球蛋白轻链激酶及其衍生肽的相互作用机制
Mechanism of 2-chloro-(epsilon-amino-Lys75)-[6-[4-(N,N- diethylamino)phenyl]-1,3,5-triazin-4-yl]calmodulin interactions with smooth muscle myosin light chain kinase and derived peptides.
作者信息
Török K, Trentham D R
机构信息
National Institute for Medical Research, Mill Hill, London, United Kingdom.
出版信息
Biochemistry. 1994 Nov 1;33(43):12807-20. doi: 10.1021/bi00209a012.
The mechanism of the interactions of 2-chloro-(epsilon-amino-Lys75)-[6-[4-(N,N-diethylamino)phenyl]- 1,3,5-triazin-4-yl]calmodulin (TA-calmodulin) with smooth muscle myosin light-chain kinase (MLCK) and two 17-residue peptides, Ac-R-R-K-W-Q-K-T-G-H-A-V-R-A-I-G-R-L-CONH2 (Trp peptide) and Tyr peptide, in which W is replaced by Y, were studied by measurements of equilibrium and transient fluorescence changes in the nanomolar range. Most reactions were carried out in 100 microM CaCl2 at ionic strength 0.15 M, pH 7.0, and 21 degrees C. In each case association of MLCK or peptide to TA-calmodulin could be described by a two-step process, a bimolecular step and an isomerization. In the case of the interaction between TA-calmodulin and Tyr peptide it was shown that the isomerization involved the binary complex of TA-calmodulin and Tyr peptide as opposed to an isomerization of either TA-calmodulin or Tyr peptide in isolation. These distinctions depended in part on development for transient kinetic experiments of a general theory to quantify relative phase amplitudes in two-step mechanisms. The kinetics for all three association reactions were then interpreted in terms of a bimolecular association (rate constants k+1 and k-1) followed by an isomerization of the binary complex (rate constants k+2 and k-2). For the interaction of TA-calmodulin and Tyr peptide, values of the rate constants are k+1, 8.8 x 10(8) M-1 s-1; k-1, 5.7 s-1; k+2, 0.38 s-1; and k-2, 0.65 s-1. The fluorescence intensities (lambda ex 365 nm, lambda ex 365 nm, lambda em > 400 nm) of TA-calmodulin, the initial binary complex of TA-calmodulin and Tyr peptide, and the isomerized binary complex are in the ratio 1:2.8:1.3. Analogous mechanisms were found for TA-calmodulin binding to Trp peptide and to MLCK, but values for the rate constants and relative fluorescence intensities of the binary complexes were generally not so completely defined. Values for the Trp peptide and MLCK, respectively, are k+1, 8.8 x 10(8) M-1 s-1 and 1.1 x 10(8) M-1 s-1; (k+2 + k-2), 0.97 s-1 and 1.3 s-1; and k-1k-2/(k+2 + k-2), 0.0079 s-1 and 0.025-0.056 s-1. Equilibrium dissociation constants (Kd) for interactions of TA-calmodulin and targets determined from these data are Tyr peptide, 4.1 nM; Trp peptide, 0.011 nM; and MLCK, 0.23-0.51 nM.(ABSTRACT TRUNCATED AT 400 WORDS)
通过测量纳摩尔范围内的平衡荧光变化和瞬态荧光变化,研究了2-氯-(ε-氨基-Lys75)-[6-[4-(N,N-二乙氨基)苯基]-1,3,5-三嗪-4-基]钙调蛋白(TA-钙调蛋白)与平滑肌肌球蛋白轻链激酶(MLCK)以及两个17残基肽(Ac-R-R-K-W-Q-K-T-G-H-A-V-R-A-I-G-R-L-CONH2(色氨酸肽)和酪氨酸肽,其中W被Y取代)之间的相互作用机制。大多数反应在100μM氯化钙、离子强度0.15M、pH7.0和21℃的条件下进行。在每种情况下,MLCK或肽与TA-钙调蛋白的结合都可以用两步过程来描述,即双分子步骤和异构化。在TA-钙调蛋白与酪氨酸肽相互作用的情况下,结果表明异构化涉及TA-钙调蛋白和酪氨酸肽的二元复合物,而不是单独的TA-钙调蛋白或酪氨酸肽的异构化。这些差异部分取决于为瞬态动力学实验开发的一种通用理论,该理论用于量化两步机制中的相对相位幅度。然后根据双分子缔合(速率常数k+1和k-1),接着是二元复合物的异构化(速率常数k+2和k-2)来解释所有三个缔合反应的动力学。对于TA-钙调蛋白与酪氨酸肽的相互作用,速率常数的值为k+1,8.8×10^8M^-1s^-1;k-1,5.7s^-1;k+2,0.38s^-1;k-2,0.65s^-1。TA-钙调蛋白、TA-钙调蛋白与酪氨酸肽的初始二元复合物以及异构化二元复合物的荧光强度(激发波长365nm,发射波长>400nm)之比为1:2.8:1.3。发现TA-钙调蛋白与色氨酸肽和MLCK结合的机制类似,但二元复合物的速率常数和相对荧光强度的值通常没有如此完整地确定。色氨酸肽和MLCK的相应值分别为k+1,8.8×10^8M^-1s^-1和1.1×10^8M^-1s^-1;(k+2 + k-2),0.97s^-1和1.3s^-1;k-1k-2/(k+2 + k-2),0.0079s^-1和0.025 - 0.056s^-1。根据这些数据确定的TA-钙调蛋白与靶标的相互作用的平衡解离常数(Kd)为:酪氨酸肽,4.1nM;色氨酸肽,0.011nM;MLCK,0.23 - 0.51nM。(摘要截断于400字)
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