首页> 美国卫生研究院文献>Journal of Bacteriology >Characterization of genes in the cellulose-synthesizing operon (acs operon) of Acetobacter xylinum: implications for cellulose crystallization.
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Characterization of genes in the cellulose-synthesizing operon (acs operon) of Acetobacter xylinum: implications for cellulose crystallization.

机译:木醋杆菌纤维素合成操纵子(acs操纵子)中的基因表征:对纤维素结晶的影响。

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摘要

The synthesis of an extracellular ribbon of cellulose in the bacterium Acetobacter xylinum takes place from linearly arranged, membrane-localized, cellulose-synthesizing and extrusion complexes that direct the coupled steps of polymerization and crystallization. To identify the different components involved in this process, we isolated an Acetobacter cellulose-synthesizing (acs) operon from this bacterium. Analysis of DNA sequence shows the presence of three genes in the acs operon, in which the first gene (acsAB) codes for a polypeptide with a molecular mass of 168 kDa, which was identified as the cellulose synthase. A single base change in the previously reported DNA sequence of this gene, resulting in a frameshift and synthesis of a larger protein, is described in the present paper, along with the sequences of the other two genes (acsC and acsD). The requirement of the acs operon genes for cellulose production was determined using site-determined TnphoA/Kanr GenBlock insertion mutants. Mutant analysis showed that while the acsAB and acsC genes were essential for cellulose production in vivo, the acsD mutant produced reduced amounts of two cellulose allomorphs (cellulose I and cellulose II), suggesting that the acsD gene is involved in cellulose crystallization. The role of the acs operon genes in determining the linear array of intramembranous particles, which are believed to be sites of cellulose synthesis, was investigated for the different mutants; however, this arrangement was observed only in cells that actively produced cellulose microfibrils, suggesting that it may be influenced by the crystallization of the nascent glucan chains.
机译:木醋杆菌中纤维素的细胞外带的合成是由线性排列的,膜定位的,纤维素合成的和挤出的复合物进行的,这些复合物指导聚合和结晶的耦合步骤。为了确定此过程中涉及的不同组件,我们从该细菌中分离出了醋杆菌纤维素合成(acs)操纵子。 DNA序列分析显示acs操纵子中存在三个基因,其中第一个基因(acsAB)编码分子量为168 kDa的多肽,被鉴定为纤维素合成酶。本文描述了该基因先前报道的DNA序列中的单个碱基变化,导致移码和合成了更大的蛋白质,以及其他两个基因(acsC和acsD)的序列。使用位点确定的TnphoA / Kanr GenBlock插入突变体确定了acs操纵子基因对纤维素生产的需求。突变分析表明,虽然acsAB和acsC基因对于体内纤维素的产生至关重要,但acsD突变体产生的两种纤维素同种异形体(纤维素I和纤维素II)的数量减少,这表明acsD基因参与了纤维素的结晶。对于不同的突变体,研究了acs操纵子基因在确定膜内颗粒的线性阵列中的作用,该膜被认为是纤维素合成的位点。然而,这种排列仅在活跃产生纤维素微纤维的细胞中观察到,表明它可能受新生葡聚糖链结晶的影响。

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