Gong Huansheng, Byers David M
Department of Pediatrics, Atlantic Research Centre, Dalhousie University, Rm C-305 Clinical Research Centre, 5849 University Avenue, Nova Scotia, Halifax, Canada B3H 4H7.
Biochem Biophys Res Commun. 2003 Feb 28;302(1):35-40. doi: 10.1016/s0006-291x(03)00108-6.
Bacterial acyl carrier protein (ACP) is a small, acidic, and highly conserved protein that supplies acyl groups for biosynthesis of a variety of lipid products. Recent modelling studies predict that residues primarily in helix II of Escherichia coli ACP (Glu-41, Ala-45) are involved in its interaction with the condensing enzyme FabH of fatty acid synthase. Using recombinant Vibrio harveyi ACP as a template for site-directed mutagenesis, we have shown that an acidic residue at position 41 is essential for V. harveyi fatty acid synthase (but not acyl-ACP synthetase) activity. In contrast, various replacements of Ala-45 were tolerated by both enzymes. None of the mutations introduced dramatic structural changes based on circular dichroism and native gel electrophoresis. These results confirm that Glu-41 of ACP is a critical residue for fatty acid synthase, but not for all enzymes that utilize ACP as a substrate.
细菌酰基载体蛋白(ACP)是一种小的、酸性的且高度保守的蛋白质,它为多种脂质产物的生物合成提供酰基。最近的模型研究预测,大肠杆菌ACP(Glu-41、Ala-45)主要在螺旋II中的残基参与其与脂肪酸合酶的缩合酶FabH的相互作用。我们以重组哈维氏弧菌ACP作为定点诱变的模板,结果表明41位的酸性残基对于哈维氏弧菌脂肪酸合酶(而非酰基-ACP合成酶)的活性至关重要。相比之下,Ala-45的各种替代对这两种酶均具有耐受性。基于圆二色性和天然凝胶电泳,所引入的突变均未引起显著的结构变化。这些结果证实,ACP的Glu-41是脂肪酸合酶的关键残基,但并非所有利用ACP作为底物的酶的关键残基。
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