DNA ISOLATION BY A RAPID METHOD FROM HUMAN BLOOD-SAMPLES - EFFECTS OF MGCL2, EDTA, STORAGE TIME, AND TEMPERATURE ON DNA YIELD AND QUALITY

被引：85

作者：

LAHIRI, DK

SCHNABEL, B

机构：

[1] Laboratory of Molecular Neurogenetics, Institute of Psychiatric Research, Department of Psychiatry, Indiana University School of Medicine, Indianapolis, Indiana

[2] Laboratory of Molecular Neurogenetics, Institute of Psychiatric Research, Indiana University School of Medicine, Indianapolis, Indiana, 46202-4887

来源：

BIOCHEMICAL GENETICS | 1993年 / 31卷 / 7-8期

关键词：

HIGH MOLECULAR WEIGHT DNA; MGCL2; INTEGRITY OF DNA; RAPID METHOD; DNA BANKING;

D O I：

10.1007/BF00553174

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

The isolation of DNA from whole blood by a modified rapid method (RM) was tested using various detergents and buffer conditions. Extraction of DNA with either NP-40 or Triton X-100 gave a high yield of undegraded DNA in less than an hour The concentration of magnesium ion in the buffers was critical to obtaining intact, high molecular weight (HMW) DNA. Greater than 10 mM MgCl2 led to degradation. Addition of EDTA to the buffer inhibits this degradation. Preparation of DNA from blood stored at room temperature or incubated at 37-degrees-C for 24 hr resulted in the same amount and quality of DNA as from samples frozen at -70-degrees-C DNA from blood samples that had undergone more than four freeze-thaw cycles was found to be partially degraded. The modified RM can be applied to extract DNA from as little as 10 mul of blood (340 ng of DNA) and from dried blood samples. DNA samples remained intact and undegraded for longer times when DNA was dissolved in higher concentrations of EDTA.

引用

页码：321 / 328

页数：8

共 10 条

[1] HUMAN GENE-THERAPY [J].

ANDERSON, WF .

SCIENCE, 1992, 256 (5058) :808-813

[2] PURIFICATION OF HUMAN-LEUKOCYTE DNA - PROTEINASE-K IS NOT NECESSARY [J].

DOUGLAS, AM ;

GEORGALIS, AM ;

BENTON, LR ;

CANAVAN, KL ;

ATCHISON, BA .

ANALYTICAL BIOCHEMISTRY, 1992, 201 (02) :362-365

[3] A NONORGANIC AND NONENZYMATIC EXTRACTION METHOD GIVES HIGHER YIELDS OF GENOMIC DNA FROM WHOLE-BLOOD SAMPLES THAN DO 9 OTHER METHODS TESTED [J].

LAHIRI, DK ;

BYE, S ;

NURNBERGER, JI ;

HODES, ME ;

CRISP, M .

JOURNAL OF BIOCHEMICAL AND BIOPHYSICAL METHODS, 1992, 25 (04) :193-205

[4] A RAPID NONENZYMATIC METHOD FOR THE PREPARATION OF HMW DNA FROM BLOOD FOR RFLP STUDIES [J].

LAHIRI, DK ;

NURNBERGER, JI .

NUCLEIC ACIDS RESEARCH, 1991, 19 (19) :5444-5444

[5] DNA BANKING - THE EFFECTS OF STORAGE OF BLOOD AND ISOLATED DNA ON THE INTEGRITY OF DNA [J].

MADISEN, L ;

HOAR, DI ;

HOLROYD, CD ;

CRISP, M ;

HODES, ME .

AMERICAN JOURNAL OF MEDICAL GENETICS, 1987, 27 (02) :379-390

[6]

Maniatis T., 1982, MOL CLONING

[7] DNA MICROEXTRACTION FROM DRIED BLOOD SPOTS ON FILTER-PAPER BLOTTERS - POTENTIAL APPLICATIONS TO NEWBORN SCREENING [J].

MCCABE, ERB ;

HUANG, SZ ;

SELTZER, WK ;

LAW, ML .

HUMAN GENETICS, 1987, 75 (03) :213-216

[8] HUMAN GENE-THERAPY COMES OF AGE [J].

MILLER, AD .

NATURE, 1992, 357 (6378) :455-460

[9] A SIMPLE SALTING OUT PROCEDURE FOR EXTRACTING DNA FROM HUMAN NUCLEATED CELLS [J].

MILLER, SA ;

DYKES, DD ;

POLESKY, HF .

NUCLEIC ACIDS RESEARCH, 1988, 16 (03) :1215-1215

[10] ANALYSIS OF ENZYMATICALLY AMPLIFIED BETA-GLOBIN AND HLA-DQ-ALPHA DNA WITH ALLELE-SPECIFIC OLIGONUCLEOTIDE PROBES [J].

SAIKI, RK ;

BUGAWAN, TL ;

HORN, GT ;

MULLIS, KB ;

ERLICH, HA .

NATURE, 1986, 324 (6093) :163-166

← 1 →