Proteomic profiling reveals crucial retinal protein alterations in the early phase of an experimental glaucoma model

Fabian Anders; Julia Teister; Sebstian Funke; Norbert Pfeiffer; Franz Grus; Thanos Solon; Verena Prokosch

doi:10.1007/s00417-017-3678-x

Proteomic profiling reveals crucial retinal protein alterations in the early phase of an experimental glaucoma model

Graefes Arch Clin Exp Ophthalmol. 2017 Jul;255(7):1395-1407. doi: 10.1007/s00417-017-3678-x. Epub 2017 May 24.

Authors

Fabian Anders¹, Julia Teister¹, Sebstian Funke¹, Norbert Pfeiffer^{1

2}, Franz Grus¹, Thanos Solon³, Verena Prokosch^{4

5}

Affiliations

¹ Experimental Ophthalmology, Department of Ophthalmology, University Medical Center, Langenbeckstrasse 1, 55131, Mainz, Germany.
² University Eye Hospital Mainz, School of Medicine, Langenbeckstrasse 1, 55131, Mainz, Germany.
³ Department of Experimental Ophthalmology, University Medical Center, Domagkstraße 15, 48149, Münster, Germany.
⁴ Experimental Ophthalmology, Department of Ophthalmology, University Medical Center, Langenbeckstrasse 1, 55131, Mainz, Germany. vprokosch@gmx.de.
⁵ University Eye Hospital Mainz, School of Medicine, Langenbeckstrasse 1, 55131, Mainz, Germany. vprokosch@gmx.de.

PMID: 28536832
DOI: 10.1007/s00417-017-3678-x

Abstract

Purpose: Clinical glaucoma is difficult to assess in terms of molecular pathophysiology, prompting studies in experimental models of glaucoma. The purpose of this study was to investigate quantitative changes in retinal protein expression at the onset of experimental glaucoma in rats. Analyzing the proteome provides a suitable tool to decipher the pathophysiological processes in glaucomatous degeneration.

Methods: Thermic cauterization of episcleral veins was utilized to elevate the intraocular pressure in Sprague Dawley rats. Morphological changes were surveyed on a cellular level with a staining of Brn3a-positive cells. The retinal nerve fiber layer was investigated using optical coherence tomography (OCT, Heidelberg Engineering) and the optic nerve was analyzed by an axonal grading system. Mass spectrometry-featured quantitative proteomics and immunohistochemical staining was used to identify specifically altered proteins in the course of intraocular pressure elevation and initial neurodegeneration. Proteomic data were further analyzed with Ingenuity Pathway Analysis and Cytoscape to analyze further molecular associations.

Results: The intraocular pressure rose significantly (p < 0.001) for the follow-up period of 3 weeks after which animals were sacrificed. Eyes exposed to an elevated intraocular pressure showed an initial decrease of retinal ganglion cells, retinal nerve fiber layer (p < 0.05) and an impairment of the optic nerve (p < 0.01). Mass spectrometry led to the identification and quantification of 931 retinal proteins, whereas 32 were considerably altered. Bioinformatics-assisted clustering revealed that a majority of these proteins are functionally associated with cell differentiation, apoptosis and stress response. The creation of an interactive protein network showed that numerous altered proteins are connected regarding their cellular function. Protein kinase b, mitogen-activated protein kinase 1 and the NF-κB complex seem to be essential molecules in this context.

Conclusions: In conclusion, these results provide further lines of evidence that substantial molecular changes occur at the onset of the disease, identifying potential key players, which might be useful as biomarkers for diagnostics and development of medical treatment in the future.

Keywords: Apoptosis; Biomarker; Electron spray ionization mass spectrometry; Glaucoma; Iron homeostasis; Protein network.

MeSH terms

Animals
Disease Models, Animal
Eye Proteins / metabolism*
Female
Glaucoma / diagnosis
Glaucoma / metabolism*
Proteomics / methods*
Rats
Rats, Sprague-Dawley
Retina / metabolism*
Retina / pathology
Tomography, Optical Coherence

Substances

Eye Proteins