首页> 美国卫生研究院文献>Journal of Bacteriology >Characterization of mutants of Caulobacter crescentus defective in surface attachment of the paracrystalline surface layer.
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Characterization of mutants of Caulobacter crescentus defective in surface attachment of the paracrystalline surface layer.

机译:新月形芽孢杆菌突变体的表征在顺晶表面层的表面附着中有缺陷。

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摘要

Strains of Caulobacter crescentus express a paracrystalline surface layer (S-layer) consisting of the protein RsaA. Mutants of C. crescentus NA1000 and CB2, isolated for their ability to grow in the absence of calcium ions, uniformly no longer had the S-layer attached to the cell surface. However, RsaA was still produced, and when colonies grown on calcium-sufficient medium were examined, large two-dimensional arrays of S-layer were found intermixed with the cells. Such arrays were not found in calcium-deficient medium even when high levels of magnesium ions were provided. The arrays could be disrupted with divalent ion chelators and more readily with the calcium-selective ethylene glycol-bis (beta-aminoethyl ether)N,N,N',N'-tetraacetic acid (EGTA). Thus, the outer membrane surface was not needed as a template for self-assembly, but calcium likely was. The cell surface and S-layer gene of assembly-defective mutants of NA1000 were examined to determine the basis of the S-layer surface attachment defect. Mutants had no detectable alteration in the rough lipopolysaccharide (LPS) or a characterized capsular polysaccharide, but another polysaccharide molecule was greatly reduced or absent in all calcium-independent mutants. The molecule was shown to be a smooth LPS with a core sugar and fatty acid complement identical to those of the rough LPS and an O polysaccharide of homogeneous length, tentatively considered to be composed of 4,6-dideoxy-4-amino hexose, 3,6-dideoxy-3-amino hexose, and glycerol in equal proportions. This molecule (termed SLPS) was detectable by surface labeling with a specific antiserum only when the S-layer was not present. The rsaA genes from three calcium-independent mutants were cloned and expressed in an S-layer-negative, SLPS-positive strain. A normal S-layer was produced, ruling out defects in rsaA in these cases. It is proposed that SLPS is required for S-layer surface attachment, possibly via calcium bridging. The data support the possibility that calcium binding is required to prevent an otherwise lethal effect of SLPS. If true, mutations that eliminate the O polysaccharide of SLPS eliminate the lethal effects of calcium-deprived SLPS, at the expense of S-layer attachment.
机译:新月形杆菌的菌株表达由蛋白质RsaA组成的同晶表面层(S层)。由于在没有钙离子的情况下生长的能力而分离的新月形梭菌NA1000和CB2突变体不再均匀地具有附着在细胞表面的S层。然而,仍然产生RsaA,并且当检查在钙充足的培养基上生长的菌落时,发现大的二维S层阵列与细胞混合。即使提供了高水平的镁离子,在缺乏钙的培养基中也找不到这种阵列。可用二价离子螯合剂破坏阵列,而用钙选择性乙二醇-双(β-氨基乙基醚)N,N,N',N'-四乙酸(EGTA)更容易破坏阵列。因此,不需要将外膜表面用作自组装的模板,但可能需要钙。检查了NA1000的装配缺陷型突变体的细胞表面和S层基因,以确定S层表面附着缺陷的基础。突变体在粗脂多糖(LPS)或特征性荚膜多糖中均未检测到变化,但在所有不依赖钙的突变体中,另一种多糖分子大大减少或缺失。该分子显示为平滑的LPS,具有与粗LPS相同的核心糖和脂肪酸补体,并且具有均一长度的O多糖,初步认为由4,6-二脱氧-4-氨基己糖3组成。 ,6-二脱氧-3-氨基己糖和甘油的比例相同。仅当不存在S层时,才可以通过表面标记特定的抗血清来检测此分子(称为SLPS)。克隆了三个不依赖钙的突变体的rsaA基因,并在S层阴性,SLPS阳性菌株中表达。产生了正常的S层,排除了这些情况下rsaA中的缺陷。建议S层表面连接可能需要SLPS,可能通过钙桥连接。数据支持需要钙结合以防止SLPS否则具有致命作用的可能性。如果为真,消除SLPS O多糖的突变消除了缺钙的SLPS的致死作用,但以S层附着为代价。

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