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荧光标记的肌球蛋白亚片段1与核苷酸及肌动蛋白的相互作用。

Interaction of fluorescently labeled myosin subfragment 1 with nucleotides and actin.

作者信息

Aguirre R, Gonsoulin F, Cheung H C

出版信息

Biochemistry. 1986 Nov 4;25(22):6827-35. doi: 10.1021/bi00370a015.

DOI:10.1021/bi00370a015
PMID:3801396
Abstract

Isolated myosin heads (subfragment 1) were modified by covalent attachment of 5-(iodoacetamido)fluorescein or 5-(iodoacetamido)salicylic acid to the essential sulfhydryl group SH1. The extrinsic fluorescence of the modified proteins was sensitive to binding of nucleotides and F-actin. With the fluorescein derivative [subfragment 1 (S1) modified with 5-(iodoacetamido)fluorescein (IAF) at SH1 (S1-AF)], association with MgADP decreased the probe fluorescence by 30%, whereas binding to actin increased the emission by a factor of 2. In the ternary complex acto-S1-AF X MgADP, the effect of nucleotide on the intensity of the attached fluorescein canceled the effect of actin. The fluorescence state of this ternary complex was similar to that of S1-AF X MgADP. The emission of S1-AF was resolved into two components with lifetimes of 4.3 and 0.6 ns and relative contributions of 33% and 67%, respectively. Interaction of S1-AF with nucleotides and actin did not alter the lifetimes but significantly shifted their fractional contributions. Quenching studies showed that the short lifetime likely arose from the fluorescein moiety statically quenched by internal groups. Binding of MgADP to the salicylate derivative [S1 modified with 5-(iodoacetamido)salicylic acid at SH1 (S1-SAL)] induced a 25% enhancement of the probe fluorescence, whereas formation of acto-S1-SAL decreased the emission by 10% regardless of whether MgADP was bound to the protein. Both labeled S1 species bound MgADP with a similar affinity, comparable to that of unmodified S1 previously reported by other investigators.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

通过将5-(碘乙酰胺基)荧光素或5-(碘乙酰胺基)水杨酸共价连接到必需的巯基SH1上,对分离的肌球蛋白头部(亚片段1)进行修饰。修饰后蛋白质的外在荧光对核苷酸和F-肌动蛋白的结合敏感。对于荧光素衍生物[在SH1处用5-(碘乙酰胺基)荧光素(IAF)修饰的亚片段1(S1)(S1-AF)],与MgADP结合使探针荧光降低30%,而与肌动蛋白结合使发射增强2倍。在三元复合物肌动蛋白-S1-AF·MgADP中,核苷酸对连接的荧光素强度的影响抵消了肌动蛋白的影响。该三元复合物的荧光状态与S1-AF·MgADP的相似。S1-AF的发射可分解为两个成分,寿命分别为4.3和0.6 ns,相对贡献分别为33%和67%。S1-AF与核苷酸和肌动蛋白的相互作用没有改变寿命,但显著改变了它们的相对贡献。猝灭研究表明,短寿命可能是由于荧光素部分被内部基团静态猝灭所致。MgADP与水杨酸盐衍生物[在SH1处用5-(碘乙酰胺基)水杨酸修饰的S1(S1-SAL)]结合导致探针荧光增强25%,而无论MgADP是否与蛋白质结合,肌动蛋白-S1-SAL的形成都会使发射降低10%。两种标记的S1物种与MgADP的结合亲和力相似,与其他研究者先前报道的未修饰S1的亲和力相当。(摘要截断于250字)

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