Implementation and evaluation of amyloidosis subtyping by laser-capture microdissection and tandem mass spectrometry

被引:63
作者
Mollee, Peter [1 ]
Boros, Samuel [2 ]
Loo, Dorothy [3 ]
Ruelcke, Jayde E. [3 ]
Lakis, Vanessa A. [3 ]
Kim-Anh Le Cao [3 ]
Renaut, Patricia [2 ]
Hill, Michelle M. [3 ]
机构
[1] Princess Alexandra Hosp, Amyloidosis Ctr, Brisbane, Qld 4102, Australia
[2] Princess Alexandra Hosp, Pathol Queensland, Dept Anat Pathol, Brisbane, Qld, Australia
[3] Univ Queensland, Diamantina Inst, Translat Res Inst, Level 5,37 Kent St, Woolloongabba, Qld 4102, Australia
基金
澳大利亚研究理事会; 英国医学研究理事会;
关键词
Amyloid; Mass spectrometry; Laser capture microdissection; Diagnosis; Proteomics; RENAL AMYLOIDOSIS; DIAGNOSIS; PROTEOMICS; BIOPSIES; CLASSIFICATION;
D O I
10.1186/s12014-016-9133-x
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
Background: Correct identification of the amyloidosis-causing protein is crucial for clinical management. Recently the Mayo Clinic reported laser-capture microdissection (LCM) with liquid chromatography-coupled tandem mass spectrometry (MS/MS) as a new diagnostic tool for amyloid diagnosis. Here, we report an independent implementation of this proteomic diagnostics method at the Princess Alexandra Hospital Amyloidosis Centre in Brisbane, Australia. Results: From 2010 to 2014, 138 biopsies received from 35 different organ sites were analysed by LCM-MS/MS using Congo Red staining to visualise amyloid deposits. There was insufficient tissue in the block for LCM for 7 cases. An amyloid forming protein was ultimately identified in 121 out of 131 attempted cases (94 %). Of the 121 successful cases, the Mayo Clinic amyloid proteomic signature (at least two of Serum Amyloid P, ApoE and ApoA4) was detected in 92 (76 %). Low levels of additional amyloid forming proteins were frequently identified with the main amyloid forming protein, which may reflect co-deposition of fibrils. Furthermore, vitronectin and clusterin were frequently identified in our samples. Adding vitronectin to the amyloid signature increases the number of positive cases, suggesting a potential 4th protein for the signature. In terms of clinical impact, amyloid typing by immunohistochemistry was attempted in 88 cases, reported as diagnostic in 39, however, 5 were subsequently revealed by proteomic analysis to be incorrect. Overall, the referring clinician's diagnosis of amyloid subtype was altered by proteomic analysis in 24 % of cases. While LCM-MS/MS was highly robust in protein identification, clinical information was still required for subtyping, particularly for systemic versus localized amyloidosis. Conclusions: This study reports the independent implementation and evaluation of a proteomics-based diagnostic for amyloidosis subtyping. Our results support LCM-MS/MS as a powerful new diagnostic technique for amyloidosis, but also identified some challenges and further development opportunities.
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页码:1 / 6
页数:6
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