Institut Pasteur, Unité Génétique Moléculaire, CNRS ERL 3526, Paris, France.
J Bacteriol. 2012 May;194(9):2142-51. doi: 10.1128/JB.06641-11. Epub 2012 Jan 27.
Lgt of Escherichia coli catalyzes the transfer of an sn-1,2-diacylglyceryl group from phosphatidylglycerol to prolipoproteins. The enzyme is essential for growth, as demonstrated here by the analysis of an lgt depletion strain. Cell fractionation demonstrated that Lgt is an inner membrane protein. Its membrane topology was determined by fusing Lgt to β-galactosidase and alkaline phosphatase and by substituted cysteine accessibility method (SCAM) studies. The data show that Lgt is embedded in the membrane by seven transmembrane segments, that its N terminus faces the periplasm, and that its C terminus faces the cytoplasm. Highly conserved amino acids in Lgt of both Gram-negative and Gram-positive bacteria were identified. Lgt enzymes are characterized by a so-called Lgt signature motif in which four residues are invariant. Ten conserved residues were replaced with alanine, and the activity of these Lgt variants was analyzed by their ability to complement the lgt depletion strain. Residues Y26, N146, and G154 are absolutely required for Lgt function, and R143, E151, R239, and E243 are important. The results demonstrate that the majority of the essential residues of Lgt are located in the membrane and that the Lgt signature motif faces the periplasm.
大肠杆菌 Lgt 催化 sn-1,2-二酰基甘油基从磷脂酰甘油转移到原脂蛋白。该酶对生长是必需的,正如这里对 lgt 耗竭菌株的分析所示。细胞分级分离表明 Lgt 是一种内膜蛋白。通过将 Lgt 与β-半乳糖苷酶和碱性磷酸酶融合以及通过取代半胱氨酸可及性方法(SCAM)研究,确定了其膜拓扑结构。数据表明,Lgt 通过七个跨膜片段嵌入膜中,其 N 端面向周质,C 端面向细胞质。鉴定了革兰氏阴性和革兰氏阳性细菌中 Lgt 的高度保守氨基酸。Lgt 酶的特征在于所谓的 Lgt 特征基序,其中四个残基是不变的。十个保守残基被丙氨酸取代,并通过它们补充 lgt 耗竭菌株的能力来分析这些 Lgt 变体的活性。残基 Y26、N146 和 G154 对 Lgt 功能绝对必需,而 R143、E151、R239 和 E243 很重要。结果表明,Lgt 的大多数必需残基位于膜中,并且 Lgt 特征基序面向周质。
