A群链球菌毒力的遗传控制。2质粒对抗吞噬活性、不透明因子及IgG和IgA fc受体的触发作用。

L A Burova, L E Ravdonikas, P Christensen, C Schalén, A A Totolian
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引用次数: 0

摘要

pSM19035和pERL1两种质粒的红霉素耐药标记可以在A群链球菌内和H群与A群链球菌之间偶联,频率为10(-5)~ 8 × 10(-7)。使用的两种受体菌株22v-1和22v-2显示不透明因子(of)活性的痕迹。这种活性在两种质粒转移到菌株后显著增加,而其他一些受体,即22h-21、12Teiko-1和Challis 6-1,在结合后仍保持of阴性。此外,以菌株22v-1和22v-2为受体的杂交接合物表达了抗吞噬活性。对这些异偶体进行了分型,但不属于M12型、M22型(亲本的来源型)M3型或M1型。在22v-1和22v-2的转接合体中,伴随着抗吞噬活性的表达,出现了IgG和IgA fc受体活性,而供体和受体细胞则没有受体。虽然它们保留了作为Emr标记物供体的能力,但不可能证明在转缀合物中具有抗吞噬、OF或fc受体活性的染色体外DNA。提示质粒触发抗吞噬活性、of、IgG和IgA fc受体可能是由于质粒DNA插入到染色体中。
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The genetic control of virulence in group A streptococci. II. Trigger effect by plasmids on anti-phagocytic activity, opacity factor and IgG and IgA Fc-receptors.

The erythromycin-resistance marker of two plasmids, pSM19035 and pERL1, could be transferred by conjugation in matings within group A streptococci and between group H and group A streptococci, with a frequency of 10(-5) to 8 X 10(-7). Two of the recipient strains used, 22v-1 and 22v-2, showed traces of opacity factor (OF) activity. This activity increased markedly upon transfer of both plasmids to the strains, whereas a number of other recipients, viz. 22h-21, 12Teiko-1 and Challis 6-1, remained OF-negative after conjugation. Furthermore, the transconjugants resulting from matings using strains 22v-1 and 22v-2 as recipients expressed anti-phagocytic activity. Attempts were made to type the transconjugants but they did not belong to type M12, M22 (the types from which the parents were derived) M3 or M1. Concomitant with the expression of anti-phagocytic activity, IgG and IgA Fc-receptor activity occurred in the transconjugants of 22v-1 and 22v-2, whereas the donor and recipient cells were without receptors. It was not possible to demonstrate extrachromosomal DNA in transconjugants possessing anti-phagocytic, OF or Fc-receptor activity, although they retained their ability to serve as donors of the Emr marker. It is suggested that the triggering by plasmids of anti-phagocytic activity, OF and IgG and IgA Fc-receptors is due to insertion of plasmid DNA into the chromosome.

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The genetic control of virulence in group A streptococci. III. Plasmid-induced "switch-off"--effect on some pathogenic properties. The microscopic diagnosis of Pneumocystis carinii. An evaluation of the gram, the methylene blue, and the Ziehl-Neelsen procedures. The genetic control of virulence in group A streptococci. II. Trigger effect by plasmids on anti-phagocytic activity, opacity factor and IgG and IgA Fc-receptors. Investigation of Micrococcaceae in a department of cardiac surgery. Biochemical characterization and sensitivity patterns of strains isolated from patients, staff, and air. Evaluation of Minibact, a new system for rapid identification of Enterobacteriaceae. Comparison of Minibact, Micro-ID and API 20E with a conventional method as reference.
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