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首页> 外文期刊>Gut: Journal of the British Society of Gastroenterology >Detection of novel non-M2-related antimitochondrial antibodies in patients with anti-M2 negative primary biliary cirrhosis.
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Detection of novel non-M2-related antimitochondrial antibodies in patients with anti-M2 negative primary biliary cirrhosis.

机译:抗M2阴性原发性胆汁性肝硬化患者中新型非M2相关的抗线粒体抗体的检测。

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摘要

OBJECTIVE: In 95% of patients with primary biliary cirrhosis (PBC) antimitochondrial antibodies (AMAs) can be detected reacting with at least one of the five components of the M2 antigen identified as the 2-oxoacid dehydrogenase complex (OADC). However, among our PBC sera 15-20% are anti-M2 negative by ELISA and western blotting but in the immunofluorescence test (IFT) they show the typical AMA staining. The aim of the present study was to characterise the target antigen(s) of these non-M2-related AMAs. PATIENTS AND METHODS: We analysed sera from 27 patients with clinically and histologically proven PBC being AMA positive by the IFT but anti-M2 negative by ELISA and western blotting. They were tested by western blotting against various 100,000 g supernatants obtained after sonication of mitochondria from rat liver, bovine heart and pig kidney. These were further separated by isopycnic sucrose density centrifugation using different sucrose density fractions. RESULTS: Fourteen of the 27 AMA positive/anti-M2 negative sera (52%) reacted in the western blotting with a 60 kDa protein and eight (29%) with an 80 kDa protein, both present in the 100 000 g supernatant from bovine heart mitochondria accumulating at sucrose densities of 1.14-1.16. An identity of these determinants with any of the M2-related antigens could be excluded. In the 60 kDa band components of the mitochondrial enzymes F(1)F(0)-ATPase, ubiquinone cytochrome c reductase and acyl CoA dehydrogenase were detected by MALDI-TOF analysis; the 80 kDa protein could not be further characterised. CONCLUSIONS: AMA positive/anti-M2 negative PBC sera contain antibodies to further mitochondrial antigens at 60 and 80 kDa which do not correspond to any of the M2 determinants. Those antibodies can be detected to a lesser extent in sera from patients with classical anti-M2 positive PBC but not in patients with other hepatic and non-hepatic disorders and may, therefore, represent additional marker antibodies for the serological diagnosis of PBC.
机译:目的:在95%的原发性胆汁性肝硬化(PBC)患者中,可以检测到抗线粒体抗体(AMAs)与M2抗原的五个成分中的至少一种反应,该成分被确定为2-氧合酸脱氢酶复合物(OADC)。然而,在我们的PBC血清中,通过ELISA和Western印迹检测到抗M2阴性的比例为15-20%,但在免疫荧光测试(IFT)中,它们显示出典型的AMA染色。本研究的目的是表征这些非M2相关AMA的靶抗原。患者和方法:我们分析了27例临床和组织学证实为PBC的患者的血清,其中IBC通过IFT检测为AMA阳性,而通过ELISA和Western印迹检测为抗M2阴性。通过蛋白质印迹对来自大鼠肝脏,牛心脏和猪肾脏的线粒体进行超声处理后获得的各种100,000 g上清液进行了测试。这些通过使用不同蔗糖密度级分的等密度蔗糖密度离心进一步分离。结果:27种AMA阳性/抗M2阴性血清中有14种(52%)在Western blotting中与60 kDa蛋白反应,八种(29%)与80 kDa蛋白反应,均存在于100000 g牛上清液中心脏线粒体的蔗糖密度为1.14-1.16。可以排除这些决定簇与任何M2相关抗原的同一性。在线粒体酶F(1)F(0)-ATPase的60 kDa条带成分中,通过MALDI-TOF分析检测了泛醌细胞色素c还原酶和酰基CoA脱氢酶; 80 kDa蛋白无法进一步表征。结论:AMA阳性/抗M2阴性的PBC血清含有针对60和80 kDa的线粒体抗原的抗体,这些抗体与任何M2决定簇都不对应。这些抗体可以从经典抗M2阳性PBC患者的血清中检出程度较低,但在其他肝和非肝疾病患者中则不能检出,因此可能代表了PBC血清学诊断的其他标志物抗体。

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