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对一株对小鼠具有毒力的M50组A链球菌菌株的emm基因簇进行DNA测序和基因表达分析。

DNA sequencing and gene expression of the emm gene cluster in an M50 group A streptococcus strain virulent for mice.

作者信息

Yung D L, Hollingshead S K

机构信息

Department of Microbiology, University of Alabama at Birmingham, USA.

出版信息

Infect Immun. 1996 Jun;64(6):2193-200. doi: 10.1128/iai.64.6.2193-2200.1996.

Abstract

The strain B514, an M serotype 50 strain, is capable of causing a natural upper respiratory infection leading to death in mice, as reported by Hook et al. in 1960 (E. W. Hook, R. R. Wagner, and R. C. Lancefield, Am. J. Hyg. 72:111-119, 1960). Thus, this strain was of interest for use in developing an animal model for group A streptococcal colonization and disease. The emm gene cluster for this strain was examined by PCR mapping and found to contain three emm family genes and cluster pattern 5. PCR-generated fragments corresponding to the SF4 (mrp50), SF2 (emmL50), and SF3 (enn50) genes were cloned and the entire gene cluster was sequenced. The gene cluster has greater than 97% DNA identity to previously sequenced regions of the gene cluster of the M2 strain T2/44/RB4 if two small divergent regions that encode the mature amino terminus of the SF-2 and SF-3 gene products are not included. If expressed, the genes encode proteins which bind human immunoglobulin G (Mrp50 and EmmL50) or immunoglobulin A (Enn50). However, in isolates taken directly after passage in mice, the surface proteins arising from these genes were barely detectable. The transcription of each gene in the B514 strain was investigated by Northern (RNA) hybridization, and mRNA transcripts were detected and quantitated relative to those of the recA gene, a housekeeping gene. Transcription of all three emm family genes was found to be over 30-fold attenuated relative to transcription of the same genes in strain T2/44/RB4. This suggests that the positive regulator, Mga, either is not expressed in this strain or has a different requirement for activation; it also suggests that the capsule may be sufficient to inhibit phagocytosis under these circumstances.

摘要

如胡克等人在1960年所报道的(E.W.胡克、R.R.瓦格纳和R.C.兰斯菲尔德,《美国卫生杂志》72:111 - 119,1960),菌株B514是M血清型50菌株,能够在小鼠中引发自然上呼吸道感染并导致死亡。因此,该菌株对于开发A组链球菌定植和疾病的动物模型具有研究价值。通过PCR图谱分析对该菌株的emm基因簇进行了检测,发现其包含三个emm家族基因且簇型为5。对应于SF4(mrp50)、SF2(emmL50)和SF3(enn50)基因的PCR扩增片段被克隆,并对整个基因簇进行了测序。如果不包括编码SF - 2和SF - 3基因产物成熟氨基末端的两个小的差异区域,该基因簇与M2菌株T2/44/RB4基因簇先前测序区域的DNA同一性大于97%。如果这些基因得以表达,它们编码的蛋白质可结合人免疫球蛋白G(Mrp50和EmmL50)或免疫球蛋白A(Enn50)。然而,在小鼠传代后直接获取的分离株中,这些基因产生的表面蛋白几乎检测不到。通过Northern(RNA)杂交研究了B514菌株中每个基因的转录情况,并相对于看家基因recA的mRNA转录本对mRNA转录物进行了检测和定量。发现所有三个emm家族基因的转录相对于T2/44/RB4菌株中相同基因的转录减弱了30倍以上。这表明正调控因子Mga要么在该菌株中不表达,要么对激活有不同的需求;这也表明在这些情况下,荚膜可能足以抑制吞噬作用。

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