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T4溶菌酶10种晶体形式中溶剂结合位点的保守性。

Conservation of solvent-binding sites in 10 crystal forms of T4 lysozyme.

作者信息

Zhang X J, Matthews B W

机构信息

Institute of Molecular Biology, Howard Hughes Medical Institute, University of Oregon, Eugene 97403.

出版信息

Protein Sci. 1994 Jul;3(7):1031-9. doi: 10.1002/pro.5560030705.

Abstract

Solvent-binding sites were compared in 10 different crystal forms of phage T4 lysozyme that were refined using data from 2.6 A to 1.7 A resolution. The sample included 18 crystallographically independent lysozyme molecules. Despite different crystallization conditions, variable crystal contacts, changes due to mutation, and varying attention to solvent during crystallographic refinement, 62% of the 20 most frequently occupied sites were conserved. Allowing for potential steric interference from neighboring molecules in the crystal lattice, this fraction increased to 79% of the sites. There was, however, no solvent-binding site that was occupied in all 18 lysozyme molecules. A buried double site was occupied in 17 instances and 2 other internal sites were occupied 15 times. Apart from these buried sites, the most frequently occupied sites were often at the amino-termini of alpha-helices. Solvent molecules at the most conserved sites tended to have crystallographic thermal factors lower than average, but atoms with low B-factors were not restricted to these sites. Although superficial inspection may suggest that only 50-60% (or less) of solvent-binding sites are conserved in different crystal forms of a protein, it appears that many sites appear to be empty either because of steric interference or because the apparent occupancy of a given site can vary from crystal to crystal. The X-ray method of identifying sites is somewhat subjective and tends to result in specification only of those solvent molecules that are well ordered and bound with high occupancy, even though there is clear evidence for solvent bound at many additional sites.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

在利用分辨率从2.6埃至1.7埃的数据精修的噬菌体T4溶菌酶的10种不同晶体形式中,对溶剂结合位点进行了比较。该样本包含18个晶体学独立的溶菌酶分子。尽管结晶条件不同、晶体接触可变、因突变而产生变化以及在晶体学精修过程中对溶剂的关注度不同,但20个最常占据的位点中有62%是保守的。考虑到晶格中相邻分子的潜在空间干扰,这一比例增加到了位点的79%。然而,没有一个溶剂结合位点在所有18个溶菌酶分子中都被占据。一个埋藏的双位点在17个实例中被占据,另外2个内部位点被占据了15次。除了这些埋藏位点外,最常占据的位点通常位于α螺旋的氨基末端。最保守位点处的溶剂分子往往具有低于平均水平的晶体学热因子,但具有低B因子的原子并不局限于这些位点。尽管初步检查可能表明,在一种蛋白质的不同晶体形式中,只有50 - 60%(或更少)的溶剂结合位点是保守的,但似乎许多位点看起来是空的,要么是由于空间干扰,要么是因为给定位点的表观占有率在不同晶体之间可能会有所不同。通过X射线方法识别位点有点主观,并且往往只会确定那些排列良好且占有率高的溶剂分子,即使有明确证据表明在许多其他位点也有溶剂结合。(摘要截断于250字)

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