Development of a droplet digital PCR assay for quantification of the proviral load of bovine leukemia virus

被引:8
|
作者
De Brun, Maria L. [1 ]
Cosme, Bruno [2 ]
Petersen, Marcos [3 ]
Alvarez, Irene [3 ,5 ]
Folgueras-Flatschart, Aurea [2 ]
Flatschart, Roberto [2 ]
Panei, Carlos Javier [4 ]
Puentes, Rodrigo [1 ]
机构
[1] Univ Republica, Inst Patobiol, Unidad Microbiol, Fac Vet, Montevideo, Uruguay
[2] Inst Nacl Metrol Calidad & Tecnol Inmetro, Rio De Janeiro, Brazil
[3] Inst Nacl Tecnol Agr INTA, Inst Virol & Innovac Tecnol IVIT, Buenos Aires, DF, Argentina
[4] Univ Nacl La Plata FCV UNLP, Lab Virol, Fac Ciencias Vet, La Plata, Argentina
[5] Consejo Nacl Invest Cient & Tecn CONICET, Buenos Aires, DF, Argentina
关键词
bovine leukemia virus; droplet digital PCR; enzootic bovine leukosis; proviral load; REAL-TIME PCR; CHAIN-REACTION; INFECTION; BLV; DNA; QUANTITATION;
D O I
10.1177/10406387221085581
中图分类号
S85 [动物医学(兽医学)];
学科分类号
0906 ;
摘要
Droplet digital PCR (ddPCR) is a highly sensitive tool developed for the detection and quantification of short-sequence variants-a tool that offers unparalleled precision enabling measurement of smaller-fold changes. We describe here the use of ddPCR for the detection of Bovine leukemia virus (BLV) DNA provirus. Serum samples and whole blood from experimentally infected sheep and naturally infected cattle were analyzed through ddPCR to detect the BLV gp51 gene, and then compared with serologic and molecular tests. The ddPCR assay was significantly more accurate and sensitive than AGID, ELISA, nested PCR, and quantitative PCR. The limit of detection of ddPCR was 3.3 copies/mu L, detecting positive experimentally infected sheep beginning at 6 d post-infection. The ddPCR methodology offers a promising tool for evaluating the BLV proviral load, particularly for the detection of low viral loads.
引用
收藏
页码:439 / 447
页数:9
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