Warning: Undefined array key "mm" in /www/wwwroot/www.ai-bt.com/si.php on line 10 Deprecated: trim(): Passing null to parameter #1 ($string) of type string is deprecated in /www/wwwroot/www.ai-bt.com/si.php on line 10 Development of long PCR techniques to analyze deletion mutations of the human hprt gene.

Literature DB >> 9726017

Development of long PCR techniques to analyze deletion mutations of the human hprt gene.

B Van Houten¹, Y Chen, J A Nicklas, I R Rainville, J P O'Neill.

Abstract

DNA primers and reaction conditions for long polymerase chain reaction amplification (PCR) of portions of the human hprt gene are presented. Use of these primers with DNA from previously defined hprt deletion mutants demonstrated production of the expected smaller size products as compared to DNA from wild type cells. These primers will be of value in the rapid analysis and subsequent sequencing of hprt deletion mutations in human cells.

Entities: Gene Species

Mesh：

Substances：

Year: 1998 PMID： 9726017 DOI： 10.1016/s0027-5107(98)00076-1

Source DB: PubMed Journal: Mutat Res ISSN： 0027-5107 Impact factor: 2.433

Keyword Cloud
Cited

6 in total

1. Mutations associated with base excision repair deficiency and methylation-induced genotoxic stress.

Authors: Robert W Sobol; David E Watson; Jun Nakamura; F Michael Yakes; Esther Hou; Julie K Horton; Joseph Ladapo; Bennett Van Houten; James A Swenberg; Kenneth R Tindall; Leona D Samson; Samuel H Wilson
Journal: Proc Natl Acad Sci U S A Date: 2002-04-30 Impact factor: 11.205

2. In vitro complementation of Tdp1 deficiency indicates a stabilized enzyme-DNA adduct from tyrosyl but not glycolate lesions as a consequence of the SCAN1 mutation.

Authors: Amy J Hawkins; Mark A Subler; Konstantin Akopiants; Jenny L Wiley; Shirley M Taylor; Ann C Rice; Jolene J Windle; Kristoffer Valerie; Lawrence F Povirk
Journal: DNA Repair (Amst) Date: 2009-02-10

Development of long PCR techniques to analyze deletion mutations of the human hprt gene.

1. Mutations associated with base excision repair deficiency and methylation-induced genotoxic stress.

2. In vitro complementation of Tdp1 deficiency indicates a stabilized enzyme-DNA adduct from tyrosyl but not glycolate lesions as a consequence of the SCAN1 mutation.

Review 3. Mitochondrial base excision repair assays.

4. Quantitative PCR-based measurement of nuclear and mitochondrial DNA damage and repair in mammalian cells.

5. Analysis of DNA damage and repair in nuclear and mitochondrial DNA of animal cells using quantitative PCR.

6. Quantitative Extra Long PCR to Detect DNA Lesions in Patients Exposed to Low Doses of Diagnostic Radiation