棘球蚴病的病理学

M. Reinehr, Charlotte Micheloud, F. Grimm, P. A. Kronenberg, Johannes Grimm, Annika Beck, J. Nell, Cordula Meyer zu Schwabedissen, Eva Furrer, B. Müllhaupt, T. Barth, P. Deplazes, A. Weber
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引用次数: 22

摘要

补充数字内容可在文本中找到。绦虫幼虫期的细粒棘球绦虫或多房棘球绦虫感染人可引起危及生命的人畜共患病:囊性棘球绦虫病(CE)和肺泡性棘球绦虫病(AE)。虽然囊性肝病变是这两种疾病的标志,但病程、预后和患者管理在这两种疾病之间存在决定性的差异。广泛和重叠的形态谱和有限的辅助工具的可用性是病理学家可靠地诊断和分型棘球蚴病的挑战。在这里,我们系统和定量地记录了临床和分子定义的棘球蚴病队列的病理谱(来自112名患者的138个标本)。使用一种新型单克隆抗体(mAbEmG3)进行免疫组织化学,包括其与mAbEm2G11的联合应用。6个形态学标准足以区分CE和AE:最小的囊肿大小(CE/AE: >2/≤2mm)和最大的囊肿大小(CE/AE: >25/≤25 mm),层合层厚度(CE/AE: >0.15/≤0.15 mm)和囊周纤维化(CE/AE: >0.6/≤0.6 mm),层合层条纹(CE/AE:中强/弱),囊肿数量(CE/AE:≤9/>9)。联合免疫组织化学与mAbEm2G11(特异性多房性大肠杆菌)和mAbEmG3(反应性AE和CE)具有相同的特异性,有时比聚合酶链反应更敏感。基于这些发现,我们开发了一种诊断算法用于棘球蚴病的鉴别诊断。综上所述,我们不仅确定了更确定的诊断棘球蚴病的方法,而且还定义了形态学标准,可以有力地区分CE和AE。我们希望我们的研究结果能够改善棘球蚴病的诊断,特别是对具有挑战性的病例的诊断,对棘球蚴病患者的治疗产生有益的影响。
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Pathology of Echinococcosis
Supplemental Digital Content is available in the text. Infection of humans by the larval stage of the tapeworms Echinococcus granulosus sensu lato or Echinococcus multilocularis causes the life-threatening zoonoses cystic echinococcosis (CE) and alveolar echinococcosis (AE). Although cystic liver lesions are a hallmark of both diseases, course, prognosis, and patients’ management decisively differ between the two. The wide and overlapping spectrum of morphologies and the limited availability of ancillary tools are challenges for pathologists to reliably diagnose and subtype echinococcosis. Here, we systematically and quantitatively recorded the pathologic spectrum in a clinically and molecularly defined echinococcosis cohort (138 specimens from 112 patients). Immunohistochemistry using a novel monoclonal antibody (mAbEmG3) was implemented, including its combined application with the mAbEm2G11. Six morphologic criteria sufficiently discriminated between CE and AE: size of smallest (CE/AE: >2/≤2 mm) and largest cyst (CE/AE: >25/≤25 mm), thickness of laminated layer (CE/AE: >0.15/≤0.15 mm) and pericystic fibrosis (CE/AE: >0.6/≤0.6 mm), striation of laminated layer (CE/AE: moderate-strong/weak), and number of cysts (CE/AE: ≤9/>9). Combined immunohistochemistry with mAbEm2G11 (E. multilocularis specific) and mAbEmG3 (reactive in AE and CE) was equally specific as and occasionally more sensitive than polymerase chain reaction. On the basis of these findings, we developed a diagnostic algorithm for the differential diagnosis of echinococcosis. In summary, we have not only identified the means to diagnose echinococcosis with greater certainty, but also defined morphologic criteria, which robustly discriminate between CE and AE. We expect our findings to improve echinococcosis diagnostics, especially of challenging cases, beneficially impacting the management of echinococcosis patients.
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