NONRADIOACTIVE DNA-PROBE AND POLYMERASE CHAIN-REACTION PROCEDURES FOR THE SPECIFIC DETECTION OF ACANTHAMOEBA

被引：22

作者：

LAI, SL ^{[1
]}

ASGARI, M ^{[1
]}

HENNEY, HR ^{[1
]}

机构：

[1] UNIV HOUSTON,DEPT BIOL,HOUSTON,TX 77204

来源：

MOLECULAR AND CELLULAR PROBES | 1994年 / 8卷 / 01期

关键词：

RDNA PROBE; BIOTINYLATED; POLYMERASE CHAIN REACTION (PCR); ACANTHAMOEBA;

D O I：

10.1006/mcpr.1994.1012

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

Acanthamoebae are potential pathogens which can cause serious infections of humans. A non-radioactive rDNA probe and polymerase chain reaction (PCR) amplification procedures which are specific, rapid, sensitive and safe for the detection of Acanthamoeba have been developed. A restriction fragment (126 bp; ArDNA-a) from a variable region of the cloned 26S rDNA unit of Acanthamoeba castellanii (from plasmid pAR2) was labelled by biotinylation. Cells and DNAs were incubated with the labelled rDNA probe to define conditions providing the highest hybridization specificity for Acanthamoeba by both colorimetric and chemiluminescent assays. Four recent isolates of Acanthamoeba, Acanthamoeba polyphaga, various bacteria, Herpes simplex virus, other eukaryotic amoebae and human cell lines, were sources of DNA for testing. The rDNA probe was found to be highly specific for Acanthamoeba and is capable of directly detecting about 250 cells without prior DNA purification. PCR primers for this unique ArDNA-a fragment have also been designed. Amplification of the targeted sequence by PCR using those primers yielded a single product which was specifically generated for Acanthamoeba template DNA and not DNA from the other control cells. This PCR procedure provided increased sensitivity with the direct detection of as few as 10 Acanthamoeba cells. © 1994 Academic Press. All rights reserved.

引用

页码：81 / 89

页数：9

共 50 条

[11] A HIGHLY SENSITIVE AND FAST NONRADIOACTIVE METHOD FOR DETECTION OF POLYMERASE CHAIN-REACTION PRODUCTS
HOLMSTROM, K
ROSSEN, L
RASMUSSEN, OF
ANALYTICAL BIOCHEMISTRY, 1993, 209 (02) : 278 - 283
[12] DETECTION OF CYTOMEGALOVIRUS BY THE POLYMERASE CHAIN-REACTION - A SIMPLE, RAPID AND SENSITIVE NONRADIOACTIVE METHOD
GREENFIELD, C
SINICKAS, V
HARRISON, LC
MEDICAL JOURNAL OF AUSTRALIA, 1991, 154 (06) : 383 - 385
[13] NONRADIOACTIVE DETECTION OF THE REARRANGED BCR ABL SEQUENCES AMPLIFIED BY POLYMERASE CHAIN-REACTION
LION, T
PRISCHL, F
HAAS, OA
PONT, J
SCHWARZMEIER, J
LEUKEMIA, 1991, 5 (02) : 156 - 159
[14] DETECTION OF UNTREATED MYCOBACTERIA BY USING POLYMERASE CHAIN-REACTION AND SPECIFIC DNA PROBES
FRIES, JWU
PATEL, RJ
PIESSENS, WF
WIRTH, DF
JOURNAL OF CLINICAL MICROBIOLOGY, 1991, 29 (08) : 1744 - 1747
[15] CONSTRUCTION OF A DNA PROBE AND DETECTION OF ACTINOBACILLUS-PLEUROPNEUMONIAE BY USING POLYMERASE CHAIN-REACTION
SIROIS, M
LEMIRE, EG
LEVESQUE, RC
JOURNAL OF CLINICAL MICROBIOLOGY, 1991, 29 (06) : 1183 - 1187
[16] Development of a polymerase chain reaction and a nonradioactive DNA probe for infectious laryngotracheitis virus
Abbas, F
Andreasen, JR
Jackwood, MW
AVIAN DISEASES, 1996, 40 (01) : 56 - 62
[17] SYNTHESIS OF A NONRADIOACTIVE HEPATITIS-B VIRUS-DNA PROBE FROM HUMAN SERUM BY THE POLYMERASE CHAIN-REACTION
RODRIGUEZFRIAS, F
ARRANZ, JA
BUTI, M
ESTEBAN, R
JARDI, R
EUROPEAN JOURNAL OF CLINICAL CHEMISTRY AND CLINICAL BIOCHEMISTRY, 1994, 32 (05): : 355 - 359
[18] DEVELOPMENT OF A PENAEUS MONODON-TYPE BACULOVIRUS (MBV) DNA-PROBE BY POLYMERASE CHAIN-REACTION AND SEQUENCE-ANALYSIS
LU, CC
TANG, KFJ
KOU, GH
CHEN, SN
JOURNAL OF FISH DISEASES, 1993, 16 (06) : 551 - 559
[19] DETECTION OF CYTOMEGALOVIRUS DNA BY THE POLYMERASE CHAIN-REACTION (PCR)
OPP, M
DOERR, HW
ARZTLICHE LABORATORIUM, 1991, 37 (03): : 75 - 78
[20] DETECTION OF LEGIONELLA WITH POLYMERASE CHAIN-REACTION AND GENE PROBE METHODS
MAHBUBANI, MH
BEJ, AK
MILLER, R
HAFF, L
DICESARE, J
ATLAS, RM
MOLECULAR AND CELLULAR PROBES, 1990, 4 (03) : 175 - 187

← 1 2 3 4 5 →