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用于制备丹磺酰化酰基载体蛋白的大肠杆菌酰基载体蛋白的化学修饰和翻译后修饰

Chemical and posttranslational modification of Escherichia coli acyl carrier protein for preparation of dansyl-acyl carrier proteins.

作者信息

Haas J A, Frederick M A, Fox B G

机构信息

Department of Biochemistry, University of Wisconsin, Madison, Wisconsin 53706, USA.

出版信息

Protein Expr Purif. 2000 Nov;20(2):274-84. doi: 10.1006/prep.2000.1293.

Abstract

Escherichia coli acyl carrier protein (ACP) contains a single tyrosine residue at position 71. The combined o-nitration of apo-ACP Y71 by tetranitromethane and reduction to 3-aminotyrosyl-apo-ACP were performed to introduce a specific site for attachment of a dansyl fluorescent label. Conditions for purification and characterization of dansylaminotyrosyl-apo-ACP are reported. Dansylaminotyrosyl-apo-ACP was enzymatically phosphopantetheinylated and acylated in vitro with an overall approximately 30% yield of purified stearoyl-dansylaminotyrosyl-ACP starting from unmodified apo-ACP. The steady-state kinetic parameters k(cat) = 22 min(-1) and K(M) = 2.7 microM were determined for reaction of stearoyl-dansylaminotyrosyl-ACP with stearoyl-ACP Delta(9)-desaturase. These results show that dansylaminotyrosyl-ACP will function well for studying binding interactions with the Delta(9)-desaturase and suggest similar possibilities for other ACP-dependent enzymes. The efficient in vivo phosphopantetheinylation of E. coli apo-ACP by coexpression with holo-ACP synthase in E. coli BL21(DE3) using fructose as the carbon source is also reported.

摘要

大肠杆菌酰基载体蛋白(ACP)在第71位含有一个单一的酪氨酸残基。通过用四硝基甲烷对脱辅基-ACP Y71进行联合邻位硝化并还原为3-氨基酪氨酰-脱辅基-ACP,以引入用于丹磺酰荧光标记附着的特定位点。报道了丹磺酰氨基酪氨酰-脱辅基-ACP的纯化和表征条件。丹磺酰氨基酪氨酰-脱辅基-ACP在体外进行酶促磷酸泛酰巯基乙胺化和酰化,从未修饰的脱辅基-ACP开始,纯化的硬脂酰-丹磺酰氨基酪氨酰-ACP的总产率约为30%。测定了硬脂酰-丹磺酰氨基酪氨酰-ACP与硬脂酰-ACP Δ9-去饱和酶反应的稳态动力学参数k(cat)=22 min(-1)和K(M)=2.7 μM。这些结果表明,丹磺酰氨基酪氨酰-ACP在研究与Δ9-去饱和酶的结合相互作用方面将发挥良好作用,并暗示了其他依赖ACP的酶也有类似的可能性。还报道了在大肠杆菌BL21(DE3)中使用果糖作为碳源与全酶-ACP合酶共表达时,大肠杆菌脱辅基-ACP在体内的高效磷酸泛酰巯基乙胺化。

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