作者
Boris Ovodenko, Agueda Rostagno, Thomas A Neubert, Vivekananda Shetty, Stefani Thomas, Austin Yang, Jeffrey Liebmann, Jorge Ghiso, Robert Ritch
发表日期
2007/4/1
期刊
Investigative ophthalmology and visual science
卷号
48
期号
4
页码范围
1447-1457
出版商
JB LIPPINCOTT CO
简介
purpose. To increase knowledge of the biochemical composition of lenticular exfoliation material (XFM) by using proteomic approaches.
methods. Anterior lens capsules from patients with and without exfoliation syndrome (XFS) were homogenized in formic acid and subjected to cyanogen bromide (CNBr) cleavage, and the pattern of chemically generated fragments was compared by SDS-PAGE after silver staining. Unique XFS bands not present in control cases were excised, digested with TPCK-trypsin, and the resultant peptides sequenced with quadrupole time-of-flight mass spectrometry (MS). In parallel experiments, CNBr-fragmented XFM was separately digested in solution with trypsin and elastase, and the resultant peptide mixture was analyzed by liquid chromatography coupled to tandem MS followed by identification through homology searches at nonredundant protein databases. Immunolocalization of the MS-identified components were performed in XFS versus control samples by using conventional immunohistochemical methods and light microscopy.
results. In addition to fibrillin-1, fibronectin, vitronectin, laminin, and amyloid P-component, which are well-known extracellular matrix and basement membrane components of XFM, the proteomic approaches identified the multifunctional protein clusterin and tissue inhibitor of metalloprotease (TIMP)-3 as well as novel molecules, among them fibulin-2, desmocollin-2, the glycosaminoglycans syndecan-3, and versican, membrane metalloproteases of the ADAM family (ad isintegrin and metalloprotease), and the initiation component of the classic complement activation pathway C1q. In all …
引用总数
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