Comparative Analysis of Human DNA Variations by Fluorescence-Based Sequencing of PCR Products

Kwok, Pui‐Yan; Carlson, Christopher; Yager, Thomas D.; Ankener, Wendy; Nickerson, Deborah A.

doi:10.1006/geno.1994.1469

Cited by 144 publications

(100 citation statements)

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“…4 The gene for CRTH2 is located in chromosome 11q12, a region showing linkage to asthma and asthma-associated phenotypes (for review see Hakonarson and Wjst 5 ). Using a sequencing strategy, 6 we have identified three novel SNPs in the CRTH2 gene and confirmed an in silico SNP dbSNP ID:rs545659), following a systematic screen of the exon, exon-intron boundary, 5Ј-and 3Ј-UTR sequences in a Chinese population.…”

Section: Introductionsupporting

confidence: 53%

“…Genomic DNAs were purified from peripheral blood mononuclear cells of each individual. For discovery of SNP markers, sequencing analyses of the human CRTH2 gene were performed initially using pooled DNA samples from 10 randomly chosen subjects (see also Kwok et al 6 ). Any sequence variants identified in this pool were then genotyped in the entire study population.…”

Section: Methodsmentioning

confidence: 99%

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Novel SNPs in a candidate gene, CRTH2, for allergic diseases

Hsu

Kuo

et al. 2002

Genes Immun

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Section: Introductionsupporting

confidence: 53%

Section: Methodsmentioning

confidence: 99%

Novel SNPs in a candidate gene, CRTH2, for allergic diseases

Hsu

Kuo

et al. 2002

Genes Immun

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“…The nucleotide/amino acid substitutions underlying the protein polymorphism of DNase I are summarized in Table 1. The results of this study demonstrated that the automated, direct cycle sequencing of double-stranded PCR products provides a highly reproducible method for identification of DNA sequence variations [14]. The isoenzyme ofphenotype 4 is focused to the IEF-PAGE gel region between those of phenotypes 1 and 2.…”

Section: Discussionmentioning

confidence: 94%

The molecular basis for genetic polymorphism of human deoxyribonuclease I: identification of the nucleotide substitution that generates the fourth allele

Yasuda¹,

Nadano²,

Takeshita³

et al. 1995

FEBS Letters

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In addition to the three alleles commonly responsible for the protein polymorphism of human deoxyribonuclease I, a mutation encoded by a fourth allele, DNASEI*4, was detected by isoelectric focusing. All 8 exons covering the entire open reading frame of the human DNase I gene were amplified by the polymerase chain reaction and subjected to direct sequencing. Only one nucleotide substitution, a C-to-G transition (CAG--~ GAG), in the codon for amino acid 9 of the mature enzyme was found. This substitution resulted in the replacement of Gin with Gin (Q9E).

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“…In the present study, 300 publicly available SNPs were characterized in the Korean population by comparative sequencing approach [Kwok et al, 1994]. Every SNP was tested in four samples: three individual samples and a pool of 21 individuals.…”

Section: Resultsmentioning

confidence: 99%

“…Allele frequencies of a pool were estimated by comparing the peak heights of the corresponding bases between heterozygous individual and a pooled DNA sample [Kwok et al, 1994]. The normalized peak height from heterozygous individual represents the signal contributed by 50% of the DNA template present that bears that of particular allele.…”

Section: Estimation Of Allele Frequency In a Poolmentioning

confidence: 99%