Sensitive and Specific Detection ofTrypanosoma vivaxUsing the Polymerase Chain Reaction
The nucleic acid probes that are currently in use detect and distinguishTrypanosoma vivaxparasites according to their geographic origin. To eliminate the need for using multiple DNA probes, a study was conducted to evaluate the suitability of a tandemly reiterated sequence which encodes aT. vivaxdia...
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| Veröffentlicht in: | Experimental parasitology 1997-02, Vol.85 (2), p.193-205 |
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| creator | Masake, Rachel A. Majiwa, Phelix A.O. Moloo, Shamshudeen K. Makau, Jackson M. Njuguna, James T. Maina, Mary Kabata, John ole-MoiYoi, Onesmo K. Nantulya, Vinand M. |
| description | The nucleic acid probes that are currently in use detect and distinguishTrypanosoma vivaxparasites according to their geographic origin. To eliminate the need for using multiple DNA probes, a study was conducted to evaluate the suitability of a tandemly reiterated sequence which encodes aT. vivaxdiagnostic antigen as a single probe for detection of this parasite. The antigen is recognized by monoclonal antibody Tv27 currently employed in antigen detection ELISA (Ag-ELISA). A genomic clone which contained a tetramer of the 832-bp cDNA sequence was isolated and shown to be more sensitive than the monomer. Oligonucleotide primers were designed based on the nucleotide sequence of the 832-bp cDNA insert and used in amplifying DNA sequences from the blood of cattle infected withT. vivaxisolates from West Africa, Kenya, and South America. The polymerase chain reaction (PCR) product of approximately 400 bp was obtained by amplification of DNA from all the isolates studied. The oligonucleotide primers also amplified DNA sequences inT. vivax-infected tsetse flies. Subsequently, PCR was evaluated for its capacity to detectT. vivaxDNA in the blood of three animals experimentally infected with the parasite.T. vivaxDNA was detectable in the blood of infected animals as early as 5 days post-infection. Blood and serum samples from the three cattle and from six other infected animals were also examined for the presence of trypanosomes andT. vivax-specific diagnostic antigen. Trypanosomes appeared in the blood 7–12 days post-challenge, while the antigenemia was evident on Days 5–20 of infection. Analysis of the data obtained in the three animals during the course of infection revealed that the buffy coat technique, Ag-ELISA, and PCR revealed infection in 42, 55, and 75% of the blood samples, respectively. PCR amplification of genomic DNA ofT. vivaxis thus superior to the Ag-ELISA in the detection ofT. vivax.More importantly, both theT. vivaxdiagnostic antigen and the gene encoding it are detectable in all theT. vivaxisolates examined from diverse areas of Africa and South America. |
| doi_str_mv | 10.1006/expr.1996.4124 |
| format | Article |
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To eliminate the need for using multiple DNA probes, a study was conducted to evaluate the suitability of a tandemly reiterated sequence which encodes aT. vivaxdiagnostic antigen as a single probe for detection of this parasite. The antigen is recognized by monoclonal antibody Tv27 currently employed in antigen detection ELISA (Ag-ELISA). A genomic clone which contained a tetramer of the 832-bp cDNA sequence was isolated and shown to be more sensitive than the monomer. Oligonucleotide primers were designed based on the nucleotide sequence of the 832-bp cDNA insert and used in amplifying DNA sequences from the blood of cattle infected withT. vivaxisolates from West Africa, Kenya, and South America. The polymerase chain reaction (PCR) product of approximately 400 bp was obtained by amplification of DNA from all the isolates studied. The oligonucleotide primers also amplified DNA sequences inT. vivax-infected tsetse flies. Subsequently, PCR was evaluated for its capacity to detectT. vivaxDNA in the blood of three animals experimentally infected with the parasite.T. vivaxDNA was detectable in the blood of infected animals as early as 5 days post-infection. Blood and serum samples from the three cattle and from six other infected animals were also examined for the presence of trypanosomes andT. vivax-specific diagnostic antigen. Trypanosomes appeared in the blood 7–12 days post-challenge, while the antigenemia was evident on Days 5–20 of infection. Analysis of the data obtained in the three animals during the course of infection revealed that the buffy coat technique, Ag-ELISA, and PCR revealed infection in 42, 55, and 75% of the blood samples, respectively. 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To eliminate the need for using multiple DNA probes, a study was conducted to evaluate the suitability of a tandemly reiterated sequence which encodes aT. vivaxdiagnostic antigen as a single probe for detection of this parasite. The antigen is recognized by monoclonal antibody Tv27 currently employed in antigen detection ELISA (Ag-ELISA). A genomic clone which contained a tetramer of the 832-bp cDNA sequence was isolated and shown to be more sensitive than the monomer. Oligonucleotide primers were designed based on the nucleotide sequence of the 832-bp cDNA insert and used in amplifying DNA sequences from the blood of cattle infected withT. vivaxisolates from West Africa, Kenya, and South America. The polymerase chain reaction (PCR) product of approximately 400 bp was obtained by amplification of DNA from all the isolates studied. The oligonucleotide primers also amplified DNA sequences inT. vivax-infected tsetse flies. Subsequently, PCR was evaluated for its capacity to detectT. vivaxDNA in the blood of three animals experimentally infected with the parasite.T. vivaxDNA was detectable in the blood of infected animals as early as 5 days post-infection. Blood and serum samples from the three cattle and from six other infected animals were also examined for the presence of trypanosomes andT. vivax-specific diagnostic antigen. Trypanosomes appeared in the blood 7–12 days post-challenge, while the antigenemia was evident on Days 5–20 of infection. Analysis of the data obtained in the three animals during the course of infection revealed that the buffy coat technique, Ag-ELISA, and PCR revealed infection in 42, 55, and 75% of the blood samples, respectively. PCR amplification of genomic DNA ofT. vivaxis thus superior to the Ag-ELISA in the detection ofT. vivax.More importantly, both theT. vivaxdiagnostic antigen and the gene encoding it are detectable in all theT. vivaxisolates examined from diverse areas of Africa and South America.</description><subject>DNA probes</subject><subject>oligonucleotide primers</subject><subject>Trypanosoma vivax</subject><issn>0014-4894</issn><issn>1090-2449</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>1997</creationdate><recordtype>article</recordtype><recordid>eNp1kE1LAzEQhoMoWKtXz_kDuya7yZIcpX5CQbEtHkOaTGykTZZkWbr_3l3r1dPAMM_LOw9Ct5SUlJDmDo5tKqmUTcloxc7QjBJJiooxeY5mhFBWMCHZJbrK-ZsQIsajGfpcQci-8z1gHSxetWC88wY_QAem8zHg6NZpaHWIOR407n2vj5vswxfudoDf4344QNIZ8GKnfcAfoH-xa3Th9D7Dzd-co83T43rxUizfnl8X98vCjE1Z0WypMIYLTsHICiTjTrqaN7UEQpxgwMcl2KZyxhpuasodFUIbq62rtg2v56g85ZoUc07gVJv8QadBUaImLWrSoiYtatIyAuIEwNiq95BUNh6CAevT-LGy0f-H_gB0bmuQ</recordid><startdate>199702</startdate><enddate>199702</enddate><creator>Masake, Rachel A.</creator><creator>Majiwa, Phelix A.O.</creator><creator>Moloo, Shamshudeen K.</creator><creator>Makau, Jackson M.</creator><creator>Njuguna, James T.</creator><creator>Maina, Mary</creator><creator>Kabata, John</creator><creator>ole-MoiYoi, Onesmo K.</creator><creator>Nantulya, Vinand M.</creator><general>Elsevier Inc</general><scope>AAYXX</scope><scope>CITATION</scope></search><sort><creationdate>199702</creationdate><title>Sensitive and Specific Detection ofTrypanosoma vivaxUsing the Polymerase Chain Reaction</title><author>Masake, Rachel A. ; Majiwa, Phelix A.O. ; Moloo, Shamshudeen K. ; Makau, Jackson M. ; Njuguna, James T. ; Maina, Mary ; Kabata, John ; ole-MoiYoi, Onesmo K. ; Nantulya, Vinand M.</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c1994-6b18cc5851ec92e945f9f35639e00f84e52e9ed62fcdc5c315f188acdadf2b653</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>1997</creationdate><topic>DNA probes</topic><topic>oligonucleotide primers</topic><topic>Trypanosoma vivax</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Masake, Rachel A.</creatorcontrib><creatorcontrib>Majiwa, Phelix A.O.</creatorcontrib><creatorcontrib>Moloo, Shamshudeen K.</creatorcontrib><creatorcontrib>Makau, Jackson M.</creatorcontrib><creatorcontrib>Njuguna, James T.</creatorcontrib><creatorcontrib>Maina, Mary</creatorcontrib><creatorcontrib>Kabata, John</creatorcontrib><creatorcontrib>ole-MoiYoi, Onesmo K.</creatorcontrib><creatorcontrib>Nantulya, Vinand M.</creatorcontrib><collection>CrossRef</collection><jtitle>Experimental parasitology</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Masake, Rachel A.</au><au>Majiwa, Phelix A.O.</au><au>Moloo, Shamshudeen K.</au><au>Makau, Jackson M.</au><au>Njuguna, James T.</au><au>Maina, Mary</au><au>Kabata, John</au><au>ole-MoiYoi, Onesmo K.</au><au>Nantulya, Vinand M.</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Sensitive and Specific Detection ofTrypanosoma vivaxUsing the Polymerase Chain Reaction</atitle><jtitle>Experimental parasitology</jtitle><date>1997-02</date><risdate>1997</risdate><volume>85</volume><issue>2</issue><spage>193</spage><epage>205</epage><pages>193-205</pages><issn>0014-4894</issn><eissn>1090-2449</eissn><abstract>The nucleic acid probes that are currently in use detect and distinguishTrypanosoma vivaxparasites according to their geographic origin. To eliminate the need for using multiple DNA probes, a study was conducted to evaluate the suitability of a tandemly reiterated sequence which encodes aT. vivaxdiagnostic antigen as a single probe for detection of this parasite. The antigen is recognized by monoclonal antibody Tv27 currently employed in antigen detection ELISA (Ag-ELISA). A genomic clone which contained a tetramer of the 832-bp cDNA sequence was isolated and shown to be more sensitive than the monomer. Oligonucleotide primers were designed based on the nucleotide sequence of the 832-bp cDNA insert and used in amplifying DNA sequences from the blood of cattle infected withT. vivaxisolates from West Africa, Kenya, and South America. The polymerase chain reaction (PCR) product of approximately 400 bp was obtained by amplification of DNA from all the isolates studied. The oligonucleotide primers also amplified DNA sequences inT. vivax-infected tsetse flies. Subsequently, PCR was evaluated for its capacity to detectT. vivaxDNA in the blood of three animals experimentally infected with the parasite.T. vivaxDNA was detectable in the blood of infected animals as early as 5 days post-infection. Blood and serum samples from the three cattle and from six other infected animals were also examined for the presence of trypanosomes andT. vivax-specific diagnostic antigen. Trypanosomes appeared in the blood 7–12 days post-challenge, while the antigenemia was evident on Days 5–20 of infection. Analysis of the data obtained in the three animals during the course of infection revealed that the buffy coat technique, Ag-ELISA, and PCR revealed infection in 42, 55, and 75% of the blood samples, respectively. PCR amplification of genomic DNA ofT. vivaxis thus superior to the Ag-ELISA in the detection ofT. vivax.More importantly, both theT. vivaxdiagnostic antigen and the gene encoding it are detectable in all theT. vivaxisolates examined from diverse areas of Africa and South America.</abstract><pub>Elsevier Inc</pub><doi>10.1006/expr.1996.4124</doi><tpages>13</tpages></addata></record> |
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| subjects | DNA probes oligonucleotide primers Trypanosoma vivax |
| title | Sensitive and Specific Detection ofTrypanosoma vivaxUsing the Polymerase Chain Reaction |
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