Monitoring Leishmania infantum Infections in Female Lutzomyia longipalpis by Using DNA Extraction on Cation Exchange Paper and PCR Pool Testing

被引:1
作者
Coutinho, Tiago Leonetti [1 ]
Lima Marson, Fernando Augusto [2 ]
Rangel, Osias [3 ]
Giorgio, Selma [4 ]
Silva, Kamila Cristina [1 ]
Levy, Carlos Emilio [1 ]
机构
[1] Univ Estadual Campinas, Fac Med Sci, Dept Clin Pathol, Microbiol Lab, BR-13083887 Campinas, SP, Brazil
[2] Sao Francisco Univ, Lab Med & Human Genet, Post Grad Program Hlth Sci, BR-12916900 Braganca Paulista, SP, Brazil
[3] Pasteur Inst, BR-01311000 Sao Paulo, SP, Brazil
[4] Univ Estadual Campinas, Biol Inst, BR-13083970 Campinas, SP, Brazil
关键词
diagnosis; epidemiology; Leishmania infantum; Lutzomyia longipalpis; minimum infection rate; polymerase chain reaction; visceral leishmaniasis; NATURAL INFECTION; ENDEMIC AREA; VISCERAL LEISHMANIASIS; PSYCHODIDAE; DIPTERA; STANDARDIZATION; PHLEBOTOMINAE; DIAGNOSIS; TERESINA; CHAGASI;
D O I
10.3390/diagnostics12112653
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
Visceral leishmaniasis remains a serious public health issue, and Brazil was among the seven countries with the highest prevalence of this disease worldwide. The measures to control this disease are not easily developed, and the improvement of its diagnosis, surveillance, and control is still needed. This study aimed to carry out the polymerase chain reaction (PCR) diagnosis of Leishmania infantum in vector samples in some municipalities of the State of Sao Paulo, which included two municipalities with human disease transmission and two with dog transmission only. Vectors were collected in traps with luminous bait. Next, they were killed at -4 degrees C and kept in 70% alcohol. Groups of ten female insects (pools) were mashed on cation exchange paper (fine cellulose phosphate with 18 mu Eq/cm(2) ionic exchange capacity) for DNA extraction. The PCR was carried out to identify the natural infection of the Leishmania genus in female Lutzomyia longipalpis (Lu. Longipalpis). Out of the 3880 Lu. longipalpis phlebotomines, 1060 were female and 2820 were male (3:1). The method used to extract the DNA in pools of ten phlebotomines and the PCR resulted in sensitivity, specificity, practicality, and faster analyses when compared to the individual analysis method. The procedure described can be used on a large scale in the leishmaniasis epidemiological surveillance, enabling a higher number of analyses and the optimization of human resources because the traditional diagnostic method is carried out via desiccation of the insect digestive system and microscopic examination, which is time-demanding and there is the need of manual skills.
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