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幽门螺杆菌毒力基因在体外和恒河猴体内的表达比较。

Comparison of Helicobacter pylori virulence gene expression in vitro and in the Rhesus macaque.

作者信息

Boonjakuakul Jenni K, Canfield Don R, Solnick Jay V

机构信息

Department of Medicine, Division of Infectious Disease, 513 Parnassus Avenue, HSE 418/Box 0654, University of California, San Francisco, San Francisco, CA 94143, USA.

出版信息

Infect Immun. 2005 Aug;73(8):4895-904. doi: 10.1128/IAI.73.8.4895-4904.2005.

Abstract

We used a quantitative real-time reverse transcriptase PCR assay to measure the transcript abundance of 46 known and putative Helicobacter pylori virulence genes, including 24 genes on the Cag pathogenicity island. The expression profile of H. pylori cells grown in vitro was also compared to expression in vivo after experimental infection of rhesus macaques. Transcript abundance in vitro (mid-log phase) ranged from about 0.004 (feoB and hpaA) to 20 (ureAB, napA, and cag25) copies/cell. Expression of most genes was repressed during the transition from logarithmic- to stationary-phase growth, but several well-characterized H. pylori virulence genes (katA, napA, vacA, and cagA) were induced. Comparison of results in the rhesus macaque with similar data from humans showed a strong correlation (r = 0.89). The relative in vivo expression in the rhesus monkey was highly correlated with in vitro expression during mid-log (r = 0.89)- and stationary (r = 0.88)-phase growth. Transcript abundance was on average three- to fourfold reduced in vivo compared to in vitro during mid-log phase. However, when compared to stationary phase, increased expression in vivo was observed for 6 of 7 genes on a contiguous portion of the pathogenicity island, several of which are thought to encode the H. pylori type IV structural pilus and its accessory proteins. These results suggest the possibility that some genes encoding the H. pylori type IV structural pilus and accessory proteins may form an operon that is induced during growth in vivo.

摘要

我们采用定量实时逆转录酶聚合酶链反应(PCR)分析法,测定了46个已知和推测的幽门螺杆菌毒力基因的转录丰度,其中包括空泡毒素相关基因(Cag)致病岛中的24个基因。我们还比较了体外培养的幽门螺杆菌细胞与恒河猴实验感染后体内的表达情况。体外(对数中期)转录丰度范围约为0.004(feoB和hpaA)至20(ureAB、napA和cag25)拷贝/细胞。大多数基因的表达在从对数生长期向稳定期转变过程中受到抑制,但几个已明确的幽门螺杆菌毒力基因(katA、napA、vacA和cagA)被诱导表达。将恒河猴的结果与人类的类似数据进行比较,显示出很强的相关性(r = 0.89)。恒河猴体内的相对表达与对数中期(r = 0.89)和稳定期(r = 0.88)的体外表达高度相关。与体外对数中期相比,体内转录丰度平均降低了三到四倍。然而,与稳定期相比,在致病岛相邻部分的7个基因中有6个在体内表达增加,其中几个基因被认为编码幽门螺杆菌IV型结构菌毛及其辅助蛋白。这些结果表明,一些编码幽门螺杆菌IV型结构菌毛和辅助蛋白的基因可能形成一个在体内生长过程中被诱导的操纵子。

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