Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR

Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR

Objective: To identify prevalence of chloroquine resistance point mutation at (Pfcrt, K76T) and (Pfmdr1, N86Y) copy number variation. Methods: SYBR Green I based real time PCR was used. One hundred and thirty-three samples were analyzed for (Pfcrt, K76T) and (Pfmdr1, N86Y) copy number from dried blo...

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Main Authors: Addimas Tajebe, Mulugeta Aemero, Kimani Francis, Gabriel Magoma
Format: Article
Language:English
Published: Wolters Kluwer Medknow Publications 2015-03-01
Series:Asian Pacific Journal of Tropical Biomedicine
Subjects:
Plasmodium falciparum
DNA copy number variation
Pfmdr1
Pfcrt
Real-time PCR
Online Access:http://www.sciencedirect.com/science/article/pii/S2221169115300083
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spelling doaj-0b53c0266bcd4e7392b0d589871545832020-11-24T21:57:49ZengWolters Kluwer Medknow PublicationsAsian Pacific Journal of Tropical Biomedicine2221-16912015-03-015320822010.1016/S2221-1691(15)30008-3Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCRAddimas Tajebe0Mulugeta Aemero1Kimani Francis2Gabriel Magoma3Pan African University Institute for Basic Sciences Innovation and Technology JKUAT, P. O. Box 62000-00200 Nairobi, KenyaUniversity of Gondar, P. O. Box 196, Gondar, EthiopiaKenya Medical Research Institute, P. O. Box 54840-00200 Nairobi, KenyaPan African University Institute for Basic Sciences Innovation and Technology JKUAT, P. O. Box 62000-00200 Nairobi, KenyaObjective: To identify prevalence of chloroquine resistance point mutation at (Pfcrt, K76T) and (Pfmdr1, N86Y) copy number variation. Methods: SYBR Green I based real time PCR was used. One hundred and thirty-three samples were analyzed for (Pfcrt, K76T) and (Pfmdr1, N86Y) copy number from dried blood spot. Parasite DNA was extracted using high pure DNA preparation kit. The amplification of DNA was done by using AccuPower 2× GreenStar™ qPCR Master mix. For quantification purpose a new primer pair was designed for 178 base pair template from complete genome sequence of Plasmodium falciparum strain 3D7 at NCBI. Absolute quantification method was used to determine the Pfmdr1-N86Y copy number variations. Standard curve was built from strain 3D7 gDNA since it has single copy of Pfmdr1 per haploid genome. The known positive controls with single and multi-copy number of Pfmdr1 gene were included in each experiment. The copy number ratio of the samples to the standard calibrator was made to obtain the fold difference among the samples with respect to copy number variation. Results: Out of 133 samples 73 (54.89%) were confirmed as mutant (Pfcrt, 76T) and the remaining 60 (45.11%) were genotyped as wild type (Pfcrt, K76). The (Pfmdr1, N86Y) copy number variation was determined for 133 clinical samples. Out of these samples 61 (45.86%) had single copy and the remaining 72 (54.14%) had multi-copy numbers higher than 1.5 copies per genome. Thirty-four (25.56%) multi-copies were between 1.5 and 2.5 copies per genome while 38 (28.57%) were more than 2.5 copies per genome. The minimum and maximum copies per genome were 0.474 and 4.741, respectively. Conclusions: The study showed high prevalence level and fixation of Pfcrt, 76T mutation after chloroquine withdrawal. The prevalence of Pfmdr1 copy number variant suggested that the presence of modulating factor for emergence of Plasmodium falciparum strains with higher copy numbers. However, the prevalence level was not statistically significant.http://www.sciencedirect.com/science/article/pii/S2221169115300083Plasmodium falciparumDNA copy number variationPfmdr1PfcrtReal-time PCR
collection DOAJ
language English
format Article
sources DOAJ
author Addimas Tajebe
Mulugeta Aemero
Kimani Francis
Gabriel Magoma
spellingShingle Addimas Tajebe
Mulugeta Aemero
Kimani Francis
Gabriel Magoma
Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR
Asian Pacific Journal of Tropical Biomedicine
Plasmodium falciparum
DNA copy number variation
Pfmdr1
Pfcrt
Real-time PCR
author_facet Addimas Tajebe
Mulugeta Aemero
Kimani Francis
Gabriel Magoma
author_sort Addimas Tajebe
title Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR
title_short Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR
title_full Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR
title_fullStr Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR
title_full_unstemmed Identification of chloroquine resistance Pfcrt-K76T and determination of Pfmdr1-N86Y copy number by SYBR Green I qPCR
title_sort identification of chloroquine resistance pfcrt-k76t and determination of pfmdr1-n86y copy number by sybr green i qpcr
publisher Wolters Kluwer Medknow Publications
series Asian Pacific Journal of Tropical Biomedicine
issn 2221-1691
publishDate 2015-03-01
description Objective: To identify prevalence of chloroquine resistance point mutation at (Pfcrt, K76T) and (Pfmdr1, N86Y) copy number variation. Methods: SYBR Green I based real time PCR was used. One hundred and thirty-three samples were analyzed for (Pfcrt, K76T) and (Pfmdr1, N86Y) copy number from dried blood spot. Parasite DNA was extracted using high pure DNA preparation kit. The amplification of DNA was done by using AccuPower 2× GreenStar™ qPCR Master mix. For quantification purpose a new primer pair was designed for 178 base pair template from complete genome sequence of Plasmodium falciparum strain 3D7 at NCBI. Absolute quantification method was used to determine the Pfmdr1-N86Y copy number variations. Standard curve was built from strain 3D7 gDNA since it has single copy of Pfmdr1 per haploid genome. The known positive controls with single and multi-copy number of Pfmdr1 gene were included in each experiment. The copy number ratio of the samples to the standard calibrator was made to obtain the fold difference among the samples with respect to copy number variation. Results: Out of 133 samples 73 (54.89%) were confirmed as mutant (Pfcrt, 76T) and the remaining 60 (45.11%) were genotyped as wild type (Pfcrt, K76). The (Pfmdr1, N86Y) copy number variation was determined for 133 clinical samples. Out of these samples 61 (45.86%) had single copy and the remaining 72 (54.14%) had multi-copy numbers higher than 1.5 copies per genome. Thirty-four (25.56%) multi-copies were between 1.5 and 2.5 copies per genome while 38 (28.57%) were more than 2.5 copies per genome. The minimum and maximum copies per genome were 0.474 and 4.741, respectively. Conclusions: The study showed high prevalence level and fixation of Pfcrt, 76T mutation after chloroquine withdrawal. The prevalence of Pfmdr1 copy number variant suggested that the presence of modulating factor for emergence of Plasmodium falciparum strains with higher copy numbers. However, the prevalence level was not statistically significant.
topic Plasmodium falciparum
DNA copy number variation
Pfmdr1
Pfcrt
Real-time PCR
url http://www.sciencedirect.com/science/article/pii/S2221169115300083
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