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在肾移植中,通过定量逆转录聚合酶链反应分析反映T细胞活化和细胞毒性的标志物的移植物内基因激活情况。

The intragraft gene activation of markers reflecting T-cell-activation and -cytotoxicity analyzed by quantitative RT-PCR in renal transplantation.

作者信息

Strehlau J, Pavlakis M, Lipman M, Maslinski W, Shapiro M, Strom T B

机构信息

Kinderklinik des Universitätskrankenhauses Hamburg-Eppendorf, Germany.

出版信息

Clin Nephrol. 1996 Jul;46(1):30-3.

PMID:8832147
Abstract

T-cell activation is the key event in the development of acute allograft rejection and precedes clinically apparent organ damage. We have performed competitive RT-PCR to quantify the intragraft gene expression for T-cell associated cytokines (IL-2, IL-4, IL-7, IL-15), CTLA4 and cytotoxic lymphocyte specific molecules to test their potential as rejection markers and to further elucidate mechanisms involved in graft rejection. RNA was isolated from snap-frozen portions of core biopsies obtained for the evaluation of graft dysfunction in 34 adults and 8 children. Reverse transcription derived cDNA was coamplified with a known amount of a competitor (a mutated target gene fragment) and normalized for the house keeping gene GAPDH. IL-2, the principal T-cell growth factor and IL-4 were not detectable in any biopsy at the time of histologically apparent rejection. Transcripts of the novel cytokine IL-15 were found in all dysfunctioning grafts and in two donor kidneys prior to reperfusion. CTLA-4, expressed in activated T-cells after costimulation by CD28 was uniformly present post transplantation, but not in the two donor kidneys. Transcripts for IL-7 (p < 0.001), IL-15 (p < 0.0005), CTLA4 (p = 0.04), granzyme B (p < 0.00015) and perforin (p < 0.0003) showed a significant correlation to acute rejection episodes. Heightened gene expression declined rapidly after initiation of rejection treatment. Fas-ligand mRNA gene expression was upregulated in both acute and chronic rejections. While this study shows that competitive RT-PCR is a reliable diagnostic tool to detect acute rejection in renal core biopsies, a future challenge will be to identify molecular markers of evolving rejections utilizing RT-PCR in sequential samples of fine needle aspirations, urine and blood.

摘要

T细胞活化是急性移植排斥反应发生过程中的关键事件,且早于临床上明显的器官损伤。我们进行了竞争性逆转录聚合酶链反应(RT-PCR),以定量移植组织中与T细胞相关的细胞因子(白细胞介素-2、白细胞介素-4、白细胞介素-7、白细胞介素-15)、细胞毒性T淋巴细胞相关抗原4(CTLA4)以及细胞毒性淋巴细胞特异性分子的基因表达,以测试它们作为排斥反应标志物的潜力,并进一步阐明移植排斥反应所涉及的机制。从34名成人和8名儿童的移植肾穿刺活检组织的速冻样本中提取RNA,这些活检组织用于评估移植肾功能障碍。逆转录得到的互补DNA(cDNA)与已知量的竞争物(一个突变的靶基因片段)共同扩增,并以内参基因甘油醛-3-磷酸脱氢酶(GAPDH)进行标准化。在组织学上明显出现排斥反应时,白细胞介素-2(主要的T细胞生长因子)和白细胞介素-4在任何活检组织中均未检测到。新型细胞因子白细胞介素-15的转录本在所有功能异常的移植肾以及两个再灌注前的供体肾中均有发现。CTLA4在CD28共刺激后在活化的T细胞中表达,移植后均有表达,但在两个供体肾中未表达。白细胞介素-7(p<0.001)、白细胞介素-15(p<0.0005)、CTLA4(p = 0.04)、颗粒酶B(p<0.00015)和穿孔素(p<0.0003)的转录本与急性排斥反应发作显著相关。排斥反应治疗开始后,基因表达升高迅速下降。Fas配体mRNA基因表达在急性和慢性排斥反应中均上调。虽然本研究表明竞争性RT-PCR是检测肾穿刺活检组织中急性排斥反应的可靠诊断工具,但未来的挑战将是利用RT-PCR在细针穿刺抽吸、尿液和血液的连续样本中识别正在发生的排斥反应的分子标志物。

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