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首页> 外文期刊>Acta crystallographica, Section D. Biological crystallography >Experimental phasing for structure determination using membrane-protein crystals grown by the lipid cubic phase method
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Experimental phasing for structure determination using membrane-protein crystals grown by the lipid cubic phase method

机译:使用脂质立方相法生长的膜蛋白晶体进行结构确定的实验定相

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摘要

Despite the marked increase in the number of membrane-protein structures solved using crystals grown by the lipid cubic phase or in meso method, only ten have been determined by SAD/MAD. This is likely to be a consequence of the technical difficulties associated with handling proteins and crystals in the sticky and viscous hosting mesophase that is usually incubated in glass sandwich plates for the purposes of crystallization. Here, a four-year campaign aimed at phasing the in meso structure of the integral membrane diacylglycerol kinase (DgkA) from Escherichia coli is reported. Heavy-atom labelling of this small hydrophobic enzyme was attempted by pre-labelling, co-crystallization, soaking, site-specific mercury binding to genetically engineered single-cysteine mutants and selenomethionine incorporation. Strategies and techniques for special handling are reported, as well as the typical results and the lessons learned for each of these approaches. In addition, an assay to assess the accessibility of cysteine residues in membrane proteins for mercury labelling is introduced. The various techniques and strategies described will provide a valuable reference for future experimental phasing of membrane proteins where crystals are grown by the lipid cubic phase method.
机译:尽管使用通过脂质立方相或内消旋方法生长的晶体解决的膜蛋白结构数量显着增加,但通过SAD / MAD只能测定十种。这可能是与处理粘性和粘性宿主中间相中的蛋白质和晶体相关的技术难题的结果,通常在玻璃夹心板中孵育以达到结晶的目的。在此,报道了一项为期四年的运动,旨在逐步分离来自大肠杆菌的整合膜二酰基甘油激酶(DgkA)的介观结构。通过预标记,共结晶,浸泡,位点特异性汞与基因工程单半胱氨酸突变体的结合以及硒代蛋氨酸的掺入,尝试对该小疏水酶进行重原子标记。报告了特殊处理的策略和技术,以及每种方法的典型结果和经验教训。此外,介绍了一种评估膜蛋白中半胱氨酸残基可及性的方法,可用于汞标记。所描述的各种技术和策略将为膜蛋白的未来实验定相提供有价值的参考,其中通过脂质立方相法生长晶体。

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