Literature DB >> 9865619

Analysis of tear proteins by one- and two-dimensional thin-layer iosoelectric focusing, sodium dodecyl sulfate electrophoresis and lectin blotting. Detection of a new component: cystatin C.

C Reitz1, W Breipohl, A Augustin, J Bours.   

Abstract

BACKGROUND: Isoelectric focusing (IEF) of tear proteins has not yet been carried out in a satisfactory way. Two-dimensional (2D) electrophoresis, especially in the combination of IEF with SDS, is able to differentiate between proteins in detail. The purpose of this study was therefore to analyze tear proteins by 1D IEF alone and in combination with a 2D pattern, and by IEF followed by lectin staining.
METHODS: Ampholines, covering a broad range from pH 3 to pH 10, were applied. After IEF, semi-dry blotting and incubation with a group II lectin and two group V lectins was performed.
RESULTS: Tear proteins could be separated into 31 single bands. Tear-specific pre-albumin (TSPA), lactoferrin, sIgA, IgG and lysozyme were found to be main components. Isoelectric points (IEPs, pls) of all proteins separated were determined by comparison with IEF standards. 2D patterns of IEF and SDS electrophoresis were obtained for the main subunit components of lactoferrin, sIgA, TSPA, and lysozyme. An additional new component of considerable concentration was focused at pI 8.6 with a subunit MW of 14 kDa. With s-WGA a component at an IEP of 5.2 was visualized, representing transferrin. With SNA, lactoferrin stained as a sharp main band at pI 5.1 with three additional weaker bands at IEPs from 4.8 to 4.9. At IEPs between 4.4 and 6.1, multiple components of sIgA were stained with MAA. The sugar specificity of transferrin at pI 5.2 was beta-GlcNAc. Lactoferrin showed glycation with NANA-alpha-2-6-Gal or NANA-alpha-2-6-GalNAc, whereas the sugar specificity of sIgA was NANA-alpha-2-3-Gal.
CONCLUSIONS: The investigative strategy applied here, including IEF alone, in combination with SDS-electrophoresis, and SDS-electrophoresis followed by lectin staining proved to be a reproducible method for tear protein analysis of hitherto unexperienced capacity. Lectin-stained bands of native tear proteins are not uniformly glycated by one sugar residue, but show various sugar specificities. IgA as a whole molecule is specifically glycated with NANA-alpha-2-3-Gal.

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Year:  1998        PMID: 9865619     DOI: 10.1007/s004170050177

Source DB:  PubMed          Journal:  Graefes Arch Clin Exp Ophthalmol        ISSN: 0721-832X            Impact factor:   3.117


  10 in total

1.  Effect of contact lenses on the protein composition in tear film: a ProteinChip study.

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Journal:  Graefes Arch Clin Exp Ophthalmol       Date:  2010-07-26       Impact factor: 3.117

Review 2.  Iron homeostasis and eye disease.

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3.  Detection of secretory IgM in tears during rhino-conjunctivitis.

Authors:  Johan Bours; Claudia Reitz; Jürgen Strobel; Winrich Breipohl
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4.  In vitro extraction of intra-corneal iron using reverse iontophoresis and vitamin C.

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Journal:  Graefes Arch Clin Exp Ophthalmol       Date:  2014-06-05       Impact factor: 3.117

5.  Identification of 491 proteins in the tear fluid proteome reveals a large number of proteases and protease inhibitors.

Authors:  Gustavo A de Souza; Lyris M F Godoy; Matthias Mann
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Review 6.  Molecular and Histopathological Changes Associated with Keratoconus.

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7.  Pathogen induced changes in the protein profile of human tears from Fusarium keratitis patients.

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9.  Tear fluid proteomics multimarkers for diabetic retinopathy screening.

Authors:  Zsolt Torok; Tunde Peto; Eva Csosz; Edit Tukacs; Agnes Molnar; Zsuzsanna Maros-Szabo; Andras Berta; Jozsef Tozser; Andras Hajdu; Valeria Nagy; Balint Domokos; Adrienne Csutak
Journal:  BMC Ophthalmol       Date:  2013-08-07       Impact factor: 2.209

Review 10.  Practical issues concerning tear protein assays in dry eye.

Authors:  Sharon D'Souza; Louis Tong
Journal:  Eye Vis (Lond)       Date:  2014-11-13
  10 in total

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