慢性病毒性肝炎患者体内针对可溶性肝抗原和 1 型肝细胞的自身免疫性肝炎特异性抗体。

Eirini I Rigopoulou, Maria Mytilinaiou, Ourania Romanidou, Christos Liaskos, George N Dalekos
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引用次数: 0

摘要

背景:非器官特异性自身抗体在慢性丙型肝炎(HCV)患者中非常普遍。其中,抗肝肾小球 1 型(LKM1)抗体--2 型自身免疫性肝炎(AIH-2)的血清学标志--在高达 11% 的 HCV 感染者中被检测到。另一方面,抗肝胞浆 1 型抗体(抗LC1)--既可与抗 LKM1 联合检测,也可单独检测--和抗可溶性肝抗原抗体(抗 SLA)一直被认为是 AIH 有用的特异性诊断标志物。然而,最近的一些研究对它们对AIH的特异性提出了质疑,这些研究表明,在HCV患者中,无论其抗LKM1状态如何,都能通过免疫沉淀法检测到抗LC1和抗SLA。本研究的目的是通过特异性酶联免疫吸附试验(ELISA),首先在一大群有或没有抗 LKM1 反应的希腊 HCV 感染者中检测抗LC1 和抗 SLA 的存在、首先,免疫沉淀检测法仅限于全球少数几个专业实验室,无法常规使用;其次,评估此类检测法是否适用于病毒性肝炎患者,因为基于此类酶联免疫吸附检测法的抗体检测尚未在大型 HCV 患者群体中进行过详细描述。检测方法采用商业 ELISA 对 138 名连续的 HCV 患者(120 名抗 LKM1 阴性,18 名抗 LKM1 阳性)进行抗LC1 和抗 SLA 检测。作为病理对照,还检测了相同数量(120 例)的抗 LKM1 血清阴性的慢性乙型肝炎病毒(HBV)感染者:结果:18 位抗 LKM(阳性)/HCV(阳性)患者中有 6 位(33%)抗 LKM1 检测呈阳性,而抗 LKM(阴性)/HCV(阳性)患者为 1/120 位(0.83%),抗 LKM1(阴性)/HBV(阳性)患者为 0/120 位(0%)(两组比较均 p <0.001)。HCV(带或不带抗LKM1)或HBV感染者均未出现抗SLA抗体:我们的研究表明,在一大批抗 LKM1 阴性的慢性乙型肝炎和丙型肝炎感染患者中,抗LC1 和抗 SLA 自身抗体无法通过常规检测方法检测出来。基于这些结果,我们认为在病毒性肝炎相关自身抗体血清学的常规实验室检测中应用抗LC1和抗SLA检测是不合理的,唯一可能的例外是抗LKM1(阳性)/HCV(阳性)患者的抗LC1筛查。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Autoimmune hepatitis-specific antibodies against soluble liver antigen and liver cytosol type 1 in patients with chronic viral hepatitis.

Autoimmune hepatitis-specific antibodies against soluble liver antigen and liver cytosol type 1 in patients with chronic viral hepatitis.

Autoimmune hepatitis-specific antibodies against soluble liver antigen and liver cytosol type 1 in patients with chronic viral hepatitis.

Background: Non-organ specific autoantibodies are highly prevalent in patients with chronic hepatitis C (HCV). Among them, anti-liver kidney microsomal type 1 (LKM1) antibody--the serological marker of type 2 autoimmune hepatitis (AIH-2)--is detected in up to 11% of the HCV-infected subjects. On the other hand, anti-liver cytosol type 1 antibodies (anti-LC1)--either in association with anti-LKM1, or in isolation--and anti-soluble liver antigen antibodies (anti-SLA) have been considered as useful and specific diagnostic markers for AIH. However, their specificity for AIH has been questioned by some recent studies, which have shown the detection of anti-LC1 and anti-SLA by immunoprecipitation assays in HCV patients irrespective of their anti-LKM1 status. The aim of the present study was to test the anti-LC1 and anti-SLA presence by specific enzyme linked immunosorbent assays (ELISAs), in a large group of Greek HCV-infected patients with or without anti-LKM1 reactivity as firstly, immunoprecipitation assays are limited to few specialized laboratories worldwide and cannot be used routinely and secondly, to assess whether application of such tests has any relevance in the context of patients with viral hepatitis since antibody detection based on such ELISAs has not been described in detail in large groups of HCV patients.

Methods: One hundred and thirty eight consecutive HCV patients (120 anti-LKM1 negative and 18 anti-LKM1 positive) were investigated for the presence of anti-LC1 and anti-SLA by commercial ELISAs. A similar number (120) of chronic hepatitis B virus (HBV) infected patients seronegative for anti-LKM1 was also tested as pathological controls.

Results: Six out of 18 (33%) anti-LKM(pos)/HCV(pos) patients tested positive for anti-LC1 compared to 1/120 (0.83%) anti-LKM(neg)/HCV(pos) patients and 0/120 (0%) of the anti-LKM1(neg)/HBV(pos) patients (p < 0.001 for both comparisons). Anti-SLA antibodies were not present in any of the HCV (with or without anti-LKM1) or HBV-infected patients.

Conclusion: We showed that anti-LC1 and anti-SLA autoantibodies are not detected by conventional assays in a large group of anti-LKM1 negative patients with chronic hepatitis B and C infections. Based on these results we cannot find any justification for the application of anti-LC1 and anti-SLA tests in the routine laboratory testing of viral hepatitis-related autoantibody serology with the only potential exception being the anti-LC1 screening in anti-LKM1(pos)/HCV(pos) patients.

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