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Literature DB >> 11687598

Heteroduplex formation in SMN gene dosage analysis.

S Ogino¹, D G Leonard, H Rennert, S Gao, R B Wilson.

Abstract

Most spinal muscular atrophy patients lack both copies of SMN1 exon 7 and most carriers have only one copy of SMN1 exon 7. We investigated the effect of SMN1/SMN2 heteroduplex formation on SMN gene dosage analysis, which is an assay to determine copy number of SMN1 exon 7 that utilizes multiplex quantitative polymerase chain reaction (PCR) with DraI digestion to differentiate SMN1 from SMN2. Heteroduplex formation in PCR is a well-described phenomenon. In addition to demonstrating the presence of heteroduplexes by sequence analysis of purified SMN1 bands, we compared the SMN1 signals in various genotype groups (total n = 260) to those in a group lacking SMN2 (n = 13), and we estimated the relative amounts of SMN1/SMN2 heteroduplexes. The SMN1 signal increased as SMN2 copy number increased despite a constant SMN1 copy number, although not all pairwise comparisons showed a statistically significant difference in the SMN1 signal. In conclusion, SMN1/SMN2 heteroduplexes form in SMN gene dosage analysis, falsely increasing the SMN1 signal. External controls for SMN gene dosage analysis should be chosen carefully with regard to SMN2 copy number. The effect of heteroduplex formation should be considered when performing quantitative multiplex PCR.

Entities: Disease Gene Species

Mesh：

Substances：

Year: 2001 PMID： 11687598 PMCID： PMC1906961 DOI： 10.1016/S1525-1578(10)60666-6

Source DB: PubMed Journal: J Mol Diagn ISSN： 1525-1578 Impact factor: 5.568

25 in total

1. Use of homoduplex ribosomal DNA spacer amplification products and heteroduplex cross-hybridization products in the identification of Salmonella serovars.

Authors: M A Jensen; R J Hubner
Journal: Appl Environ Microbiol Date: 1996-08 Impact factor: 4.792

2. Limitations imposed by heteroduplex formation on quantitative RT-PCR.

Authors: W N Henley; K E Schuebel; D A Nielsen
Journal: Biochem Biophys Res Commun Date: 1996-09-04 Impact factor: 3.575

3. Deletions of bases in one strand of duplex DNA, in contrast to single-base mismatches, produce highly kinked molecules: possible relevance to the folding of single-stranded nucleic acids.

Authors: C H Hsieh; J D Griffith
Journal: Proc Natl Acad Sci U S A Date: 1989-07 Impact factor: 11.205

4. Analysis of IGF2 gene imprinting in breast and colorectal cancer by allele specific-PCR.

Authors: K Yun; H Soejima; A E Merrie; J L McCall; A E Reeve
Journal: J Pathol Date: 1999-04 Impact factor: 7.996

5. Identification of proximal spinal muscular atrophy carriers and patients by analysis of SMNT and SMNC gene copy number.

Authors: P E McAndrew; D W Parsons; L R Simard; C Rochette; P N Ray; J R Mendell; T W Prior; A H Burghes
Journal: Am J Hum Genet Date: 1997-06 Impact factor: 11.025

6. Effect of PCR conditions on the formation of heteroduplex and single-stranded DNA products in the amplification of bacterial ribosomal DNA spacer regions.

Authors: M A Jensen; N Straus
Journal: PCR Methods Appl Date: 1993-12

Review 7. An update of the mutation spectrum of the survival motor neuron gene (SMN1) in autosomal recessive spinal muscular atrophy (SMA).

Authors: B Wirth
Journal: Hum Mutat Date: 2000 Impact factor: 4.878

8. Analysis of the mRNA transcripts of the survival motor neuron (SMN) gene in the tissue of an SMA fetus and the peripheral blood mononuclear cells of normals, carriers and SMA patients.

Authors: Y J Jong; J G Chang; S P Lin; T Y Yang; J C Wang; C P Chang; C C Lee; H Li; H M Hsieh-Li; C H Tsai
Journal: J Neurol Sci Date: 2000-02-15 Impact factor: 3.181

Heteroduplex formation in SMN gene dosage analysis.

1. Use of homoduplex ribosomal DNA spacer amplification products and heteroduplex cross-hybridization products in the identification of Salmonella serovars.

2. Limitations imposed by heteroduplex formation on quantitative RT-PCR.

3. Deletions of bases in one strand of duplex DNA, in contrast to single-base mismatches, produce highly kinked molecules: possible relevance to the folding of single-stranded nucleic acids.

4. Analysis of IGF2 gene imprinting in breast and colorectal cancer by allele specific-PCR.

5. Identification of proximal spinal muscular atrophy carriers and patients by analysis of SMNT and SMNC gene copy number.

6. Effect of PCR conditions on the formation of heteroduplex and single-stranded DNA products in the amplification of bacterial ribosomal DNA spacer regions.

Review 7. An update of the mutation spectrum of the survival motor neuron gene (SMN1) in autosomal recessive spinal muscular atrophy (SMA).

8. Analysis of the mRNA transcripts of the survival motor neuron (SMN) gene in the tissue of an SMA fetus and the peripheral blood mononuclear cells of normals, carriers and SMA patients.

9. A novel function for SMN, the spinal muscular atrophy disease gene product, in pre-mRNA splicing.

10. Structure and organization of the human survival motor neurone (SMN) gene.

1. SMN dosage analysis and risk assessment for spinal muscular atrophy.

2. Quantification of PCR bias caused by a single nucleotide polymorphism in SMN gene dosage analysis.

3. Spinal muscular atrophy genetic testing experience at an academic medical center.

4. Robust quantification of the SMN gene copy number by real-time TaqMan PCR.