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通过转座子Tn916插入构建血清型b特异性多糖抗原缺陷的伴放线放线杆菌突变体。

Construction of mutants of Actinobacillus actinomycetemcomitans defective in serotype b-specific polysaccharide antigen by insertion of transposon Tn916.

作者信息

Sato S, Takamatsu N, Okahashi N, Matsunoshita N, Inoue M, Takehara T, Koga T

机构信息

Department of Dental Research, National Institute of Health, Tokyo, Japan.

出版信息

J Gen Microbiol. 1992 Jun;138(6):1203-9. doi: 10.1099/00221287-138-6-1203.

DOI:10.1099/00221287-138-6-1203
PMID:1326593
Abstract

Mutants of Actinobacillus actinomycetemcomitans strain Y4 defective in the capsular-like serotype b-specific polysaccharide antigen (SPA) were constructed by inserting the transposon Tn916. Southern blot analysis suggested that the transposon was inserted into a variety of different sites on the chromosome. Whole cells from two mutants (strains ST1 and ST2) lacked reactivity with a monoclonal antibody to SPA of A. actinomycetemcomitans Y4 (mAb S5) in enzyme-linked immunosorbent assay, but those from another nine mutants (e.g. strains ST3 and ST5) reacted very weakly with mAb S5. Immunodiffusion tests showed that mAb S5 or rabbit antiserum against whole cells of strain Y4 produced a fused precipitin band with purified SPA and autoclaved extract from strain Y4, but no precipitin band with autoclaved extracts from these four mutants. The hydrolysate of autoclaved extract from strain Y4 contained equal amounts of rhamnose and fucose, component sugars of SPA. The hydrolysates of autoclaved extracts from strains ST1 and ST2 contained a trace amount of rhamnose, but not fucose. Those of autoclaved extracts from strains ST3 and ST5 contained a trace amount of fucose, but not rhamnose. All of these SPA-defective mutants reacted with a mAb to lipopolysaccharide of strain Y4. The cell hydrophobicity of SPA-defective mutants was higher than that of the parent strain. These mutant clones will be useful for analysing the gene complex responsible for the synthesis of SPA of A. actinomycetemcomitans and the regulation of expression of the polysaccharide.

摘要

通过插入转座子Tn916构建了伴放线放线杆菌Y4菌株中与类荚膜b型特异性多糖抗原(SPA)缺陷相关的突变体。Southern印迹分析表明,转座子插入到染色体上的各种不同位点。在酶联免疫吸附测定中,来自两个突变体(菌株ST1和ST2)的全细胞与抗伴放线放线杆菌Y4的SPA单克隆抗体(mAb S5)缺乏反应性,但来自另外九个突变体(如菌株ST3和ST5)的全细胞与mAb S5反应非常弱。免疫扩散试验表明,mAb S5或抗Y4菌株全细胞的兔抗血清与纯化的SPA和Y4菌株的高压灭菌提取物产生融合沉淀带,但与这四个突变体的高压灭菌提取物没有沉淀带。Y4菌株高压灭菌提取物的水解产物含有等量的鼠李糖和岩藻糖,这是SPA的组成糖。ST1和ST2菌株高压灭菌提取物的水解产物含有微量的鼠李糖,但不含岩藻糖。ST3和ST5菌株高压灭菌提取物的水解产物含有微量的岩藻糖,但不含鼠李糖。所有这些SPA缺陷突变体都与抗Y4菌株脂多糖的单克隆抗体发生反应。SPA缺陷突变体的细胞疏水性高于亲本菌株。这些突变体克隆将有助于分析负责伴放线放线杆菌SPA合成的基因复合体以及多糖表达的调控。

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