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脂多糖与溶菌酶的相互作用。脂多糖与溶菌酶的结合及对溶菌酶酶活性的抑制。

Lipopolysaccharide interaction with lysozyme. Binding of lipopolysaccharide to lysozyme and inhibition of lysozyme enzymatic activity.

作者信息

Ohno N, Morrison D C

机构信息

Department of Microbiology, Molecular Genetics and Immunology, University of Kansas Medical Center, Kansas City 66103.

出版信息

J Biol Chem. 1989 Mar 15;264(8):4434-41.

PMID:2647736
Abstract

Experiments have been carried out to characterize the binding of lysozyme (LZM) to bacteriol lipopolysaccharide (LPS). The formation of LPS.LZM complexes can be readily demonstrated using either physical-chemical separation techniques or a radiolabeled photoaffinity LPS probe. The binding affinity of LZM for LPS has been estimated to be approximately 10(8) liters/mol. Binding of LPS results in loss of LZM enzymatic activity by a noncompetitive inhibition, as assessed by either particulate or soluble substrates. This interaction of LPS with LZM is dictated primarily by hydrophobic interactions and appears to be a general property of both constituents. Binding can be demonstrated with LZM of both human and avian sources, as well as with LPS isolated from a variety of Gram-negative organisms. The addition of LPS to biologically relevant fluids containing LZM results in dose-dependent inhibition of LZM enzymatic activity suggesting that such interactions may have relevance in Gram-negative infections. Finally LZM has been shown to reduce the endotoxic activity of LPS as assessed by gelation of Limulus amoebocyte lysates.

摘要

已开展实验以表征溶菌酶(LZM)与细菌脂多糖(LPS)的结合。使用物理化学分离技术或放射性标记的光亲和性LPS探针,均可轻易证明LPS-LZM复合物的形成。据估计,LZM对LPS的结合亲和力约为10⁸升/摩尔。通过颗粒状或可溶性底物评估,LPS的结合会通过非竞争性抑制导致LZM酶活性丧失。LPS与LZM的这种相互作用主要由疏水相互作用决定,似乎是这两种成分的普遍特性。人和禽类来源的LZM以及从多种革兰氏阴性生物中分离出的LPS均可证明存在结合。向含有LZM的生物相关液体中添加LPS会导致LZM酶活性呈剂量依赖性抑制,这表明此类相互作用可能与革兰氏阴性菌感染有关。最后,通过鲎变形细胞溶解物的凝胶化评估表明,LZM已被证明可降低LPS的内毒素活性。

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