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利用激光微切割和质谱法检测膜性肾病抗原的可靠临床检测方法。

A reliable clinical test for detection of membranous nephropathy antigens using laser microdissection and mass spectrometry.

机构信息

Department of Laboratory Medicine and Pathology, Mayo Clinic, Rochester, Minnesota, USA.

Mayo Clinic Proteomics Core, Mayo Clinic, Rochester, Minnesota, USA.

出版信息

Kidney Int. 2024 Nov;106(5):907-912. doi: 10.1016/j.kint.2024.07.031. Epub 2024 Aug 26.

DOI:10.1016/j.kint.2024.07.031
PMID:39197586
Abstract

Membranous nephropathy (MN) results from accumulation of antigen-antibody immune complexes along the subepithelial region of the glomerular basement membranes. Over the last years, 13 target antigens have been discovered and include PLA2R, THSD7A, EXT1 and EXT2, NELL1, SEMA3B, NCAM1, CNTN1, HTRA1, FAT1, PCDH7, NTNG1, PCSK6 and NDNF, accounting for 80-90% of MN antigens. MN associated with many of these antigens have distinctive clinicopathologic findings. It is important to accurately identify the antigen in MN. Immunohistochemical (IHC) and/or immunofluorescence (IF) methods are currently used to detect PLA2R, THSD7A, NELL1, SEMA3B and EXT1/EXT2. However, for the remaining antigens, IHC/IF methods do not exist and are not practical for detection. Here, we developed laser microdissection-based mass spectrometry methodology (LMD/MS) as a one-stop clinical test for the detection of MN antigens using paraffin-embedded kidney biopsy tissue. The LMD/MS test was validated in two steps. LMD/MS was used to detect the antigen in 75 cases of MN with known antigens and correctly identified the antigen in all these cases. Next, LMD/MS was used to identify the antigen in 61 MN cases where the antigen was unknown and identified one of the known antigens in 40 of 61 cases including many of the less common antigens. This lower-than-expected detection rate is explained by intentional enrichment of the cohort with PLA2R-negative MN. Overall, PLA2R was identified in 16.4%, one of the other antigens detected in 49.1%, and in the remaining 34.5% of cases, none of the above antigens was detected. Thus, LMD/MS is an extremely useful and reliable method for the detection of known MN antigens and possibly indicating an unknown MN antigen for eventual discovery.

摘要

膜性肾病 (MN) 是由于抗原-抗体免疫复合物在肾小球基底膜的上皮下区域积聚而引起的。在过去的几年中,已经发现了 13 种靶抗原,包括 PLA2R、THSD7A、EXT1 和 EXT2、NELL1、SEMA3B、NCAM1、CNTN1、HTRA1、FAT1、PCDH7、NTNG1、PCSK6 和 NDNF,占 MN 抗原的 80-90%。与许多这些抗原相关的 MN 具有独特的临床病理表现。准确识别 MN 中的抗原非常重要。免疫组织化学 (IHC) 和/或免疫荧光 (IF) 方法目前用于检测 PLA2R、THSD7A、NELL1、SEMA3B 和 EXT1/EXT2。然而,对于其余的抗原,不存在 IHC/IF 方法,并且不适合检测。在这里,我们开发了基于激光微切割的质谱法 (LMD/MS),作为一种使用石蜡包埋肾活检组织检测 MN 抗原的一站式临床检测方法。LMD/MS 测试分两步进行验证。LMD/MS 用于检测 75 例已知抗原的 MN 中的抗原,并在所有这些病例中正确鉴定了抗原。接下来,LMD/MS 用于鉴定 61 例抗原未知的 MN 病例,在 61 例病例中的 40 例中鉴定出一种已知抗原,其中包括许多较少见的抗原。这种低于预期的检测率是由于有意富集 PLA2R 阴性 MN 队列所致。总体而言,在 16.4%的病例中鉴定出 PLA2R,在 49.1%的病例中检测到一种其他抗原,在其余 34.5%的病例中未检测到上述任何一种抗原。因此,LMD/MS 是一种非常有用和可靠的方法,可用于检测已知的 MN 抗原,并可能表明未知的 MN 抗原最终会被发现。

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