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马里冈比亚按蚊的杀虫剂抗性特征分析

Characterizing the insecticide resistance of Anopheles gambiae in Mali.

作者信息

Cisse Moussa B M, Keita Chitan, Dicko Abdourhamane, Dengela Dereje, Coleman Jane, Lucas Bradford, Mihigo Jules, Sadou Aboubacar, Belemvire Allison, George Kristen, Fornadel Christen, Beach Raymond

机构信息

PMI Africa Indoor Residual Spraying Project, Abt Associates, Mali, Cite du Niger. BP: 34, Bamako, Mali.

National Malaria Control Programme, Badalabougou, Rue 108 Porte 106, Bamako, Mali.

出版信息

Malar J. 2015 Aug 22;14:327. doi: 10.1186/s12936-015-0847-4.

Abstract

BACKGROUND

The impact of indoor residual spraying (IRS) and long-lasting insecticide nets (LLINs), key components of the national malaria control strategy of Mali, is threatened by vector insecticide resistance. The objective of this study was to assess the level of insecticide resistance in Anopheles gambiae sensu lato populations from Mali against four classes of insecticide recommended for IRS: organochlorines (OCs), pyrethroids (PYs), carbamates (CAs) and organophosphates (OPs). Characterization of resistance was done in 13 sites across southern Mali and assessed presence and distribution of physiological mechanisms that included target-site modifications: knockdown resistance (kdr) and altered acetycholinesterase (AChE), and/or metabolic mechanisms: elevated esterases, glutathione S-transferases (GSTs), and monooxygenases.

METHODS

The World Health Organization (WHO) tube test was used to determine phenotypic resistance of An. gambiae s.l. to: dichlorodiphenyltrichloroethane (DDT) (OC), deltamethrin (PY), lambda-cyhalothrin (PY), bendiocarb (CA), and fenitrothion (OP). Identification of sibling species and presence of the ace-1 (R) and Leu-Phe kdr, resistance-associated mutations, were determined using polymerase chain reaction (PCR) technology. Biochemical assays were conducted to detect increased activity of GSTs, oxidases and esterases.

RESULTS

Populations tested showed high levels of resistance to DDT in all 13 sites, as well as increased resistance to deltamethrin and lambda-cyhalothrin in 12 out of 13 sites. Resistance to fenitrothion and bendiocarb was detected in 1 and 4 out of 13 sites, respectively. Anopheles coluzzii, An. gambiae sensu stricto and Anopheles arabiensis were identified with high allelic frequencies of kdr in all sites where each of the species were found (13, 12 and 10 sites, respectively). Relatively low allelic frequencies of ace-1 (R) were detected in four sites where this assessment was conducted. Evidence of elevated insecticide metabolism, based on oxidase, GSTs and esterase detoxification, was also documented.

CONCLUSION

Multiple insecticide-resistance mechanisms have evolved in An. coluzzii, An. gambiae s.s. and An. arabiensis in Mali. These include at least two target site modifications: kdr, and ace-1 (R) , as well as elevated metabolic detoxification systems (monooxygenases and esterases). The selection pressure for resistance could have risen from the use of these insecticides in agriculture, as well as in public health. Resistance management strategies, based on routine resistance monitoring to inform insecticide-based malaria vector control in Mali, are recommended.

摘要

背景

室内滞留喷洒(IRS)和长效驱虫蚊帐(LLINs)是马里国家疟疾控制策略的关键组成部分,但其效果受到病媒对杀虫剂产生抗性的威胁。本研究的目的是评估马里冈比亚按蚊复合种群对推荐用于室内滞留喷洒的四类杀虫剂的抗性水平:有机氯类(OCs)、拟除虫菊酯类(PYs)、氨基甲酸酯类(CAs)和有机磷类(OPs)。在马里南部的13个地点进行了抗性特征分析,并评估了生理机制的存在和分布情况,这些生理机制包括靶标位点修饰:击倒抗性(kdr)和乙酰胆碱酯酶(AChE)改变,和/或代谢机制:酯酶、谷胱甘肽S-转移酶(GSTs)和单加氧酶活性升高。

方法

采用世界卫生组织(WHO)药管法测定冈比亚按蚊复合种群对以下杀虫剂的表型抗性:滴滴涕(OC)、溴氰菊酯(PY)、氯氟氰菊酯(PY)、残杀威(CA)和杀螟硫磷(OP)。使用聚合酶链反应(PCR)技术鉴定同胞种以及抗性相关突变ace-1(R)和亮氨酸-苯丙氨酸kdr的存在情况。进行生化测定以检测GSTs、氧化酶和酯酶活性的增加。

结果

在所有13个地点测试的种群对滴滴涕均表现出高抗性水平,并且在13个地点中的12个地点对溴氰菊酯和氯氟氰菊酯的抗性也有所增加。在13个地点中,分别有1个和4个地点检测到对杀螟硫磷和残杀威的抗性。在发现每种按蚊的所有地点(分别为所有13个地点、12个地点和10个地点),均检测到科氏按蚊、冈比亚按蚊指名亚种和阿拉伯按蚊具有较高频率的kdr等位基因。在进行此项评估的4个地点检测到相对较低频率的ace-1(R)等位基因。还记录了基于氧化酶、GSTs和酯酶解毒作用的杀虫剂代谢增强的证据。

结论

马里的科氏按蚊、冈比亚按蚊指名亚种和阿拉伯按蚊已经进化出多种抗杀虫剂机制。这些机制包括至少两种靶标位点修饰:kdr和ace-1(R),以及代谢解毒系统增强(单加氧酶和酯酶)。抗性的选择压力可能源于这些杀虫剂在农业以及公共卫生领域的使用。建议采取基于常规抗性监测的抗性管理策略,以便为马里基于杀虫剂的疟疾媒介控制提供信息。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5e99/4546276/0f1004fa279c/12936_2015_847_Fig1_HTML.jpg

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