Diagnostic PCR with Leishmania donovani specificity using sequences from the variable region of kinetoplast minicircle DNA

被引：20

作者：

Singh, N

Curran, MD

Rastogil, AK

Middleton, D

Sundar, S

机构：

[1] Cent Drug Res Inst, Div Biochem, Lucknow 226001, Uttar Pradesh, India

[2] Belfast City Hosp, No Ireland Reg Tissue Typing Lab, Belfast BT9 7AD, Antrim, North Ireland

[3] Banaras Hindu Univ, Inst Med Sci, Varanasi 221005, Uttar Pradesh, India

来源：

TROPICAL MEDICINE & INTERNATIONAL HEALTH | 1999年 / 4卷 / 06期

关键词：

Kala azar; India; Leishmania donovani; PCR; kinetoplast DNA minicircles;

D O I：

10.1046/j.1365-3156.1999.00416.x

中图分类号：

R1 [预防医学、卫生学];

学科分类号：

1004 ; 120402 ;

摘要：

Kala azar or visceral leishmaniasis, a parasitic disease caused by Leishmania donovani, is presently causing an epidemic in the eastern region of India. Diagnosis of kala azar is often complicated. We developed. a pair of oligonucleotides suitable as primers from the variable region of a predominant sequence class of minicircles of L. donovani. These primers were used in a nonisotopic polymerase chain reaction and found to be highly specific for the parasites of L. donovani complex. Using these primers, amplification of L. donovani kinetoplast DNA minicircle from the peripheral blood of kala azar patients results in a product of 204 bp. The patient group was comprised of individuals from a highly endemic region of India. We feel that PCR could assess the efficacy of new leishmanicidal drugs under investigation in these patients. PCR could also predict response to therapy which would be useful for both clinical anti research applications.

引用

页码：448 / 453

页数：6

共 12 条

[1] Andresen K, 1997, TROP MED INT HEALTH, V2, P440
[2] Bhattacharyya R, 1996, FEMS MICROBIOL LETT, V135, P195
[3] VISCERAL LEISHMANIASIS UNRESPONSIVE TO ANTIMONIAL DRUGS .1. CLINICAL AND IMMUNOLOGICAL STUDIES
BRYCESON, ADM
CHULAY, JD
HO, M
MUGAMBII, M
WERE, JB
MUIGAI, R
CHUNGE, C
GACHIHI, G
MEME, J
ANABWANI, G
BHATT, SM
[J]. TRANSACTIONS OF THE ROYAL SOCIETY OF TROPICAL MEDICINE AND HYGIENE, 1985, 79 (05) : 700 - 704
[4] QUANTITATION OF PARASITEMIA BY COMPETITIVE POLYMERASE CHAIN-REACTION AMPLIFICATION OF PARASITE KDNA MINICIRCLES DURING CHRONIC INFECTION WITH TRYPANOSOMA-CRUZI
CENTURIONLARA, A
BARRETT, L
VANVOORHIS, WC
[J]. JOURNAL OF INFECTIOUS DISEASES, 1994, 170 (05) : 1334 - 1339
[5] DIAGNOSIS OF NEW-WORLD LEISHMANIASIS - SPECIFIC DETECTION OF SPECIES OF THE LEISHMANIA-BRAZILIENSIS COMPLEX BY AMPLIFICATION OF KINETOPLAST DNA
DEBRUIJN, MHL
BARKER, DC
[J]. ACTA TROPICA, 1992, 52 (01) : 45 - 58
[6] DEBRUJIN MHL, 1993, TROP MED PARASITOL, V44, P201
[7] A SIMPLE SALTING OUT PROCEDURE FOR EXTRACTING DNA FROM HUMAN NUCLEATED CELLS
MILLER, SA
DYKES, DD
POLESKY, HF
[J]. NUCLEIC ACIDS RESEARCH, 1988, 16 (03) : 1215 - 1215
[8] AMPLIFICATION OF KINETOPLAST DNA AS A TOOL IN THE DETECTION AND DIAGNOSIS OF LEISHMANIA
RODGERS, MR
POPPER, SJ
WIRTH, DF
[J]. EXPERIMENTAL PARASITOLOGY, 1990, 71 (03) : 267 - 275
[9] RODRIGUEZ N, 1994, J CLIN MICROBIOL, V32, P2246
[10] RAPID AND SENSITIVE DETECTION OF LEISHMANIA KINETOPLAST DNA FROM SPLEEN AND BLOOD-SAMPLES OF KALA-AZAR PATIENTS
SMYTH, AJ
GHOSH, A
HASSAN, MQ
BASU, D
DEBRUIJN, MHL
ADHYA, S
MALLIK, KK
BARKER, DC
[J]. PARASITOLOGY, 1992, 105 : 183 - 192

← 1 2 →