Literature DB >> 22974592

Quantification of type II procollagen splice forms using alternative transcript-qPCR (AT-qPCR).

Audrey McAlinden1, Kyu-Hwan Shim, Louisa Wirthlin, Soumya Ravindran, Thomas M Hering.   

Abstract

During skeletal development, the onset of chondrogenic differentiation is marked by expression of the α1(II) procollagen (Col2a1) gene. Exon 2 of Col2a1 codes for a cysteine-rich von Willebrand factor C-like domain. Chondroprogenitors express the exon 2-containing IIA and IID splice forms by utilizing adjacent 5' splice sites separated by 3 base pairs. There is a shift to expression of the shorter, exon 2-lacking IIB splice form with further differentiation. Alternative splicing analysis of Col2a1 splice forms has often relied upon semi-quantitative PCR, using a single set of PCR primers to amplify multiple splice forms. We show that this widely used method is inaccurate due to mismatched amplification efficiency of different-sized PCR products. We have developed the TaqMan®-based AT-qPCR (Alternative Transcript-qPCR) assay to more accurately quantify alternatively spliced mRNA, and demonstrate the measurement of Col2a1 splice form expression in differentiating ATDC5 cells in vitro, and in wild type mouse embryonic and postnatal cartilage in vivo. The AT-qPCR assay is based on the use of a multiple-amplicon standard (MAS) plasmid, containing a chemically synthesized cluster of splice site-spanning PCR amplicons, to quantify alternative splice forms by standard curve-based qPCR. The MAS plasmid designed for Col2a1 also contained an 18S rRNA amplicon for sample normalization, and an amplicon corresponding to a region spanning exon 52-53 to measure total Col2a1 mRNA. In mouse E12.5 to P70 cartilages, we observed the expected switch between the IIA and IIB splice forms; no IID or IIC splice products were observed. However, in the ATDC5 cultures, predominant expression of the IIA and IID splice forms was found at all times in culture. Additionally, we observed that the sum of the IIA, IIB and IID splice forms comprises only a small fraction of Col2a1 transcripts containing the constitutive exon 52-53 junction. We conclude from our results that the majority of ATDC5 cells in the assay described in this study remained as chondroprogenitors during culture in standard differentiation conditions, and that additional Col2a1 transcripts may be present. The validity of this novel AT-qPCR assay was confirmed by demonstrating the expected Col2a1 isoform expression patterns in vivo in developing mouse cartilage. The ability to measure true levels of procollagen type II splice forms will provide better monitoring of chondrocyte differentiation in other model systems. In addition, the AT-qPCR assay described here could be applied to any gene of interest to detect and quantify known and predicted alternative splice forms and can be scaled up for high throughput assays.
Copyright © 2012 Elsevier B.V. All rights reserved.

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Year:  2012        PMID: 22974592      PMCID: PMC3536491          DOI: 10.1016/j.matbio.2012.08.002

Source DB:  PubMed          Journal:  Matrix Biol        ISSN: 0945-053X            Impact factor:   11.583


  53 in total

1.  Disruption of the developmentally-regulated Col2a1 pre-mRNA alternative splicing switch in a transgenic knock-in mouse model.

Authors:  Renate Lewis; Soumya Ravindran; Louisa Wirthlin; Geoffrey Traeger; Russell J Fernandes; Audrey McAlinden
Journal:  Matrix Biol       Date:  2012-01-09       Impact factor: 11.583

Review 2.  Divide, accumulate, differentiate: cell condensation in skeletal development revisited.

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4.  Effects of retinoic acid on the differentiation of chondrogenic progenitor cells, ATDC5.

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6.  Differential expression of a cysteine-rich domain in the amino-terminal propeptide of type II (cartilage) procollagen by alternative splicing of mRNA.

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  7 in total

1.  Disruption of the developmentally-regulated Col2a1 pre-mRNA alternative splicing switch in a transgenic knock-in mouse model.

Authors:  Renate Lewis; Soumya Ravindran; Louisa Wirthlin; Geoffrey Traeger; Russell J Fernandes; Audrey McAlinden
Journal:  Matrix Biol       Date:  2012-01-09       Impact factor: 11.583

2.  Characterization of a murine type IIB procollagen-specific antibody.

Authors:  Debabrata Patra; Elizabeth DeLassus; Audrey McAlinden; Linda J Sandell
Journal:  Matrix Biol       Date:  2013-11-07       Impact factor: 11.583

3.  Changes in type II procollagen isoform expression during chondrogenesis by disruption of an alternative 5' splice site within Col2a1 exon 2.

Authors:  Thomas M Hering; Louisa Wirthlin; Soumya Ravindran; Audrey McAlinden
Journal:  Matrix Biol       Date:  2014-04-13       Impact factor: 11.583

Review 4.  Alternative splicing of type II procollagen: IIB or not IIB?

Authors:  Audrey McAlinden
Journal:  Connect Tissue Res       Date:  2014-04-18       Impact factor: 3.417

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Journal:  Sci Rep       Date:  2018-07-26       Impact factor: 4.379

6.  Global Gene Expression Profiling and Alternative Splicing Events during the Chondrogenic Differentiation of Human Cartilage Endplate-Derived Stem Cells.

Authors:  Jin Shang; Xin Fan; Lei Shangguan; Huan Liu; Yue Zhou
Journal:  Biomed Res Int       Date:  2015-11-15       Impact factor: 3.411

7.  A Novel missense mutation of COL2A1 gene in a large family with stickler syndrome type I.

Authors:  Xiuzhen Liu; Hongliang Dong; Yuerong Gong; Lianqing Wang; Ruyi Zhang; Tihua Zheng; Yuxi Zheng; Shuang Shen; Chelsea Zheng; Mingming Tian; Naiguo Liu; Xiaolin Zhang; Qing Yin Zheng
Journal:  J Cell Mol Med       Date:  2022-01-21       Impact factor: 5.310

  7 in total

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