大肠杆菌中的膜结合溶菌内转糖基酶。
Membrane-bound lytic endotransglycosylase in Escherichia coli.
作者信息
Kraft A R, Templin M F, Höltje J V
机构信息
Abteilung Biochemie, Max-Planck-Institut für Entwicklungsbiologie, Tübingen, Germany.
出版信息
J Bacteriol. 1998 Jul;180(13):3441-7. doi: 10.1128/JB.180.13.3441-3447.1998.
Abstract
The gene for a novel endotype membrane-bound lytic transglycosylase, emtA, was mapped at 26.7 min of the E. coli chromosome. EmtA is a lipoprotein with an apparent molecular mass of 22kDa. Overexpression of the emtA gene did not result in bacteriolysis in vivo, but the enzyme was shown to hydrolyze glycan strands isolated from murein by amidase treatment. The formation of tetra- and hexasaccharides, but no disaccharides, reflects the endospecificity of the enzyme. The products are characterized by the presence of 1,6-anhydromuramic acid, indicating a lytic transglycosylase reaction mechanism. EmtA may function as a formatting enzyme that trims the nascent murein strands produced by the murein synthesis machinery into proper sizes, or it may be involved in the formation of tightly controlled minor holes in the murein sacculus to facilitate the export of bulky compounds across the murein barrier.
摘要
一种新型内型膜结合溶菌转糖基酶(EmtA)的基因定位于大肠杆菌染色体的26.7分钟处。EmtA是一种表观分子量为22kDa的脂蛋白。emtA基因的过表达在体内并未导致细菌溶解,但该酶可水解经酰胺酶处理后从胞壁质中分离出的聚糖链。四糖和六糖的形成,而非二糖的形成,反映了该酶的内切特异性。产物的特征是存在1,6 - 脱水胞壁酸,表明其具有溶菌转糖基酶反应机制。EmtA可能作为一种格式化酶,将胞壁质合成机制产生的新生胞壁质链修剪成合适大小,或者它可能参与在胞壁质囊泡中形成严格控制的小孔,以促进大分子化合物穿过胞壁质屏障的输出。
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