کد مقاله کد نشریه سال انتشار مقاله انگلیسی نسخه تمام متن
4011307 1602620 2012 9 صفحه PDF دانلود رایگان
عنوان انگلیسی مقاله ISI
Novel method for the rapid isolation of RPE cells specifically for RNA extraction and analysis
موضوعات مرتبط
علوم زیستی و بیوفناوری ایمنی شناسی و میکروب شناسی ایمونولوژی و میکروب شناسی (عمومی)
پیش نمایش صفحه اول مقاله
Novel method for the rapid isolation of RPE cells specifically for RNA extraction and analysis
چکیده انگلیسی

RPE cells are involved in the pathogenesis of many retinal diseases. Accurate analysis of RPE gene expression profiles in different scenarios will increase our understanding of disease mechanisms. Our objective in this study was to develop an improved method for the isolation of RPE cells, specifically for RNA analysis. Mouse RPE cells were isolated using different techniques, including mechanical dissociation techniques and a new technique we refer to here as “Simultaneous RPE cell Isolation and RNA Stabilization” (SRIRS method). RNA was extracted from the RPE cells. An RNA bioanalyzer was used to determine the quantity and quality of RNA. qPCR was used to determine contamination with non-RPE-derived RNA. Several parameters with a potential impact on the isolation protocol were studied and optimized. A marked improvement in the quantity and quality of RPE-derived RNA was obtained with the SRIRS technique. We could get the RPE in direct contact with the RNA protecting agent within 1 min of enucleation, and the RPE isolated within 11 min of enucleation. There was no significant contamination with vascular, choroidal or scleral-derived RNA. We have developed a fast, easy and reliable method for the isolation of RPE cells that leads to a high yield of RPE-derived RNA while preserving its quality. We believe this technique will be useful for future studies looking at gene expression profiles of RPE cells and their role in the pathophysiology of retinal diseases.


► We describe a new method to isolate RPE cells for gene expression analysis.
► The new method simultaneously isolates the RPE cells and stabilizes the RNA.
► RNA is protected from degradation within 1 min of enucleation.
► There is no significant contamination from non-RPE tissues.
► This method is fast, simple, reproducible and leads to high yield and quality of RNA.

ناشر
Database: Elsevier - ScienceDirect (ساینس دایرکت)
Journal: Experimental Eye Research - Volume 102, September 2012, Pages 1–9
نویسندگان
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