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OLIGONUCLEOTIDE PRIMER SEQUENCES FOR THE SPECIFIC AND SENSITIVE DETECTION OF BEBESIA BIGEMINA BY POLYMERASE CHAIN REACTION
OLIGONUCLEOTIDE PRIMER SEQUENCES FOR THE SPECIFIC AND SENSITIVE DETECTION OF BEBESIA BIGEMINA BY POLYMERASE CHAIN REACTION
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机译:聚合酶链反应特异性和灵敏检测双歧杆菌的寡核苷酸引物序列
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摘要
5" TTCCCACACGGTAGCGCGCAAAA 3"(Forward primer) and 5" GGGCGGTGAAAAGAGCAACGACA 3" (Reverse primer) for the sensitive and specific detection of B. bigemina by PCR method. The primer set was designed and custom synthesi/ed to amplify a single DNA band of 40()bp. The dc novo primers used in the PCR assay were designed using the nucleotide sequence information obtained from a monomorphic DNA fragment amplified by arbitrary primer- polymerase chain reaction from Indian isolates of Bahesia bigemina. The nucleotide sequence data comparison of this product revealed no homology with any known nucleotide sequence information of proto/oan parasites or the common mammalian host species lor the target parasite. The sensitivity limit of the primer set was 5 picograms of template DNA and higher than the previously described primer sequence (Figueroa el c;/.1992). No cross-amplification was evident with heterologous DNAs such as, bovine / hubaline leucocyte DNA and genomic DNAs obtained from common protozoan parasites of bovids like, Theileria annulata, Tryptinosoma cvansi. and Toxoplasma gondii.
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