Literature DB >> 28817123

Evaluation of telomere length in human cardiac tissues using cardiac quantitative FISH.

Maryam Sharifi-Sanjani1, Alan K Meeker2, Foteini Mourkioti1,3,4.   

Abstract

Telomere length has been correlated with various diseases, including cardiovascular disease and cancer. The use of currently available telomere-length measurement techniques is often restricted by the requirement of a large amount of cells (Southern-based techniques) or the lack of information on individual cells or telomeres (PCR-based methods). Although several methods have been used to measure telomere length in tissues as a whole, the assessment of cell-type-specific telomere length provides valuable information on individual cell types. The development of fluorescence in situ hybridization (FISH) technologies enables the quantification of telomeres in individual chromosomes, but the use of these methods is dependent on the availability of isolated cells, which prevents their use with fixed archival samples. Here we describe an optimized quantitative FISH (Q-FISH) protocol for measuring telomere length that bypasses the previous limitations by avoiding contributions from undesired cell types. We have used this protocol on small paraffin-embedded cardiac-tissue samples. This protocol describes step-by-step procedures for tissue preparation, permeabilization, cardiac-tissue pretreatment and hybridization with a Cy3-labeled telomeric repeat complementing (CCCTAA)3 peptide nucleic acid (PNA) probe coupled with cardiac-specific antibody staining. We also describe how to quantify telomere length by means of the fluorescence intensity and area of each telomere within individual nuclei. This protocol provides comparative cell-type-specific telomere-length measurements in relatively small human cardiac samples and offers an attractive technique to test hypotheses implicating telomere length in various cardiac pathologies. The current protocol (from tissue collection to image procurement) takes ∼28 h along with three overnight incubations. We anticipate that the protocol could be easily adapted for use on different tissue types.

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Year:  2017        PMID: 28817123      PMCID: PMC7716275          DOI: 10.1038/nprot.2017.082

Source DB:  PubMed          Journal:  Nat Protoc        ISSN: 1750-2799            Impact factor:   13.491


  59 in total

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Journal:  Nucleic Acids Res       Date:  1998-08-15       Impact factor: 16.971

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Journal:  Science       Date:  2011-06-30       Impact factor: 47.728

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Journal:  Eur J Heart Fail       Date:  2012-10-03       Impact factor: 15.534

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Journal:  Am J Pathol       Date:  2004-05       Impact factor: 4.307

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Journal:  J Cell Biol       Date:  1999-02-22       Impact factor: 10.539

Review 9.  Gender and telomere length: systematic review and meta-analysis.

Authors:  Michael Gardner; David Bann; Laura Wiley; Rachel Cooper; Rebecca Hardy; Dorothea Nitsch; Carmen Martin-Ruiz; Paul Shiels; Avan Aihie Sayer; Michelangela Barbieri; Sofie Bekaert; Claus Bischoff; Angela Brooks-Wilson; Wei Chen; Cyrus Cooper; Kaare Christensen; Tim De Meyer; Ian Deary; Geoff Der; Ana Diez Roux; Annette Fitzpatrick; Anjum Hajat; Julius Halaschek-Wiener; Sarah Harris; Steven C Hunt; Carol Jagger; Hyo-Sung Jeon; Robert Kaplan; Masayuki Kimura; Peter Lansdorp; Changyong Li; Toyoki Maeda; Massimo Mangino; Tim S Nawrot; Peter Nilsson; Katarina Nordfjall; Giuseppe Paolisso; Fu Ren; Karl Riabowol; Tony Robertson; Goran Roos; Jan A Staessen; Tim Spector; Nelson Tang; Brad Unryn; Pim van der Harst; Jean Woo; Chao Xing; Mohammad E Yadegarfar; Jae Yong Park; Neal Young; Diana Kuh; Thomas von Zglinicki; Yoav Ben-Shlomo
Journal:  Exp Gerontol       Date:  2013-12-21       Impact factor: 4.032

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Authors:  Richard M Cawthon
Journal:  Nucleic Acids Res       Date:  2009-01-07       Impact factor: 16.971

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