Diagnosing Salmonella enterica Serovar Typhi Infections by Polymerase Chain Reaction Using EDTA Blood Samples of Febrile Patients From Burkina Faso

被引:11
作者
Al-Emran, Hassan M. [1 ,2 ]
Hahn, Andreas [1 ]
Baum, Jana [3 ]
Espinoza, Ligia Maria Cruz [3 ]
Deerin, Jessica [3 ]
Im, Justin [3 ]
Ibrango, Samuel [4 ]
Kabore, Leon Parfait [5 ]
von Kalckreuth, Vera [3 ]
Konings, Frank [3 ]
Marks, Florian [3 ]
Sampo, Emmanuel [5 ]
Panzner, Ursula [3 ]
Park, Se Eun [3 ]
Pak, Gi Deok [3 ]
Schuett-Gerowitt, Heidi [3 ,6 ]
Vinnemeier, Christof David [3 ,7 ]
Warren, Michelle [3 ]
Soura, Abdramane Bassiahi [5 ]
机构
[1] Bernhard Nocht Inst Trop Med, Bernhard Nocht Str 74, D-20359 Hamburg, Germany
[2] German Ctr Infect Res, Hamburg, Germany
[3] Int Vaccine Inst, Seoul, South Korea
[4] Minist Hlth, Ouagadougou, Burkina Faso
[5] Univ Ouagadougou, Inst Super Sci Populat, Ouagadougou, Burkina Faso
[6] Univ Cologne, Inst Med Microbiol, Cologne, Germany
[7] Univ Med Ctr Hamburg Eppendorf, Dept Med, Hamburg, Germany
基金
比尔及梅琳达.盖茨基金会;
关键词
Burkina Faso; Salmonella; Typhi; PCR; sensitivity; BONE-MARROW; CULTURE; FEVER; PCR; BACTERIA; CHILDREN;
D O I
10.1093/cid/civ770
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Methods.aEuro integral From April 2012 to September 2013, typhoid fever surveillance was conducted in Polesgo and Nioko, 2 dry slum areas in Ouagadougou, Burkina Faso. Blood culture was performed for febrile patients using an automated blood culture system. Additional blood was collected in EDTA tubes from those patients and preserved at -80A degrees C. DNA was extracted from EDTA blood and PCR was performed to identify presence of S. Typhi. Randomly selected PCR products were further sequenced to identify S. Typhi-specific amplicons. Results.aEuro integral Of 1674 patients, S. Typhi was isolated from 18 (1.1%) individuals by blood culture. EDTA blood was collected from 1578 patients, of which 298 EDTA samples were tested by PCR. Salmonella Typhi-specific DNA was identified in 44 (14.8%) samples. The sensitivity of S. Typhi-specific PCR from EDTA blood was 89% (74%-100%) among the blood culture-positive cases. Sixteen S. Typhi-positive PCR products were sequenced, and 13 retrieved the sequence of a S. Typhi-specific amplicon. Conclusions.aEuro integral These findings suggest that blood culture-based diagnoses of S. Typhi underestimate the burden of typhoid fever in Burkina Faso. PCR could be considered as an alternative method for the identification and diagnosis of S. Typhi in blood samples.
引用
收藏
页码:S37 / S41
页数:5
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