Functional characterization of rs2229094

Functional characterization of rs2229094

Purpose: The objective of this study is to determine the expression and localization of lymphotoxin alpha (LTA) in human retinas and the functionality of one of its polymorphisms rs2229094 (C13R) (T>C), previously associated with proliferative vitreoretinopathy (PVR) development. Materials and me...

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Bibliographic Details
Published in:Clinical ophthalmology (Auckland, N.Z.) Vol. 11; p. 973
Main Authors: RodrfguezHernandez, Irene, Delgado-Tirado, Santiago, Pastor-Idoate, Salvador, GonzalezSarmiento, Rogelio, Pastor, Jose C, Rojas, Jimena, Lopez, Jose Carlos, Gonzalez-Buendia, Lucia
Format: Journal Article
Language:English
Published: Dove Medical Press Limited 01-01-2017
Subjects:
Analysis
Cytokines
Genetic polymorphisms
Inflammation
Proliferative vitreoretinopathy
Retinal detachment
Risk factors
Tumor necrosis factor
Spain
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Summary:Purpose: The objective of this study is to determine the expression and localization of lymphotoxin alpha (LTA) in human retinas and the functionality of one of its polymorphisms rs2229094 (C13R) (T>C), previously associated with proliferative vitreoretinopathy (PVR) development. Materials and methods: Total RNA from three healthy human retinas were extracted and subjected to reverse transcription-polymerase chain reaction (RT-PCR) analysis, using flanking primers of LTA cDNA. In addition, three human eyes with retinal detachment (RD) and three healthy control eyes were subjected to immunohistochemistry (IHC) with a specific antibody against LTA. The functionality of T and C alleles was assessed by using pCEFL-Flag expression vector and transient transfection assays in COS-1 cell line. In addition, expression analysis by RT-PCR, Western blot and subcellular localization of both alleles and by immunofluorescence assay was performed. Results: RT-PCR analysis revealed no significant levels of messenger RNA (mRNA) LTA in healthy human retinas. Sequential IHC staining showed differences between healthy human and RD retinas. No differences in mRNA and protein expression levels and in subcellular localization between both alleles were found. Both alleles were located in the cytoplasm of COS-1 cells. Conclusion: Although results suggest lack of functionality, the differences found in IHC study and its strong association with PVR and its relationship with tumor necrosis factor locus, warrant further studies and could justify the use of this polymorphism as a valid biomarker to identify high-risk patients to develop PVR after RD. Keywords: proliferative vitreoretinopathy, lymphotoxin alpha, tumor necrosis factor alpha, inflammation, cytokines, polymorphism
ISSN:1177-5483