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  <controlfield tag="001">INLIS000000000018044</controlfield>
  <controlfield tag="005">20220210100337</controlfield>
  <datafield tag="035" ind1=" " ind2=" ">
   <subfield code="a">0010-0222000018</subfield>
  </datafield>
  <controlfield tag="007">ta</controlfield>
  <controlfield tag="008">220210                |          | |  </controlfield>
  <datafield tag="100" ind1="1" ind2=" ">
   <subfield code="a">Ekawasti, Fitrine</subfield>
  </datafield>
  <datafield tag="245" ind1="1" ind2=" ">
   <subfield code="a">Restriction fragment length polymorphism analysis of genes of virulent  strain isolate of Toxoplasma gondii using enzyme DdeI /</subfield>
   <subfield code="c">Ekawasti, Fitrine</subfield>
  </datafield>
  <datafield tag="260" ind1=" " ind2=" ">
   <subfield code="c">2021</subfield>
  </datafield>
  <datafield tag="300" ind1=" " ind2=" ">
   <subfield code="a">7(2):196-203</subfield>
  </datafield>
  <datafield tag="650" ind1=" " ind2="4">
   <subfield code="a">DdeI, genotype, restriction enzyme, Toxoplasma gondii.</subfield>
  </datafield>
  <datafield tag="700" ind1="1" ind2=" ">
   <subfield code="a">Cahyaningsih, Umi</subfield>
  </datafield>
  <datafield tag="700" ind1="1" ind2=" ">
   <subfield code="a">Dharmayanti, NLP Indi</subfield>
  </datafield>
  <datafield tag="700" ind1="1" ind2=" ">
   <subfield code="a">Saâ€™diah, Siti</subfield>
  </datafield>
  <datafield tag="700" ind1="1" ind2=" ">
   <subfield code="a">Subekti, Didik Tulus</subfield>
  </datafield>
  <datafield tag="700" ind1="1" ind2=" ">
   <subfield code="a">Azmi, Zul</subfield>
  </datafield>
  <datafield tag="700" ind1="1" ind2=" ">
   <subfield code="a">Desem, Muhammad Ibrahim</subfield>
  </datafield>
  <datafield tag="520" ind1=" " ind2=" ">
   <subfield code="a">Background and Aim: Toxoplasma gondii is a unicellular coccidian parasite distributed globally and is an important &#13;
zoonotic pathogen. Approximately 30% of the human population worldwide is chronically infected with T. gondii. The &#13;
pathogenicity of this species depends on the type originating from the clonal population. Techniques for more accurately &#13;
determining the type of T. gondii have recently been developed using genetic markers. Specifically, T. gondii has been typed &#13;
using polymerase chain reaction-restriction fragment length polymorphism (PCR-RFLP). This study aimed to identify sets &#13;
of PCR-RFLP markers that have high power to discriminate genotyping of T. gondii and are easy to use and are easy to use. &#13;
The objective of this study was to characterize virulent strain isolates of T. gondii by PCR-RFLP using 10 markers with &#13;
DdeI.&#13;
&#13;
Materials and Methods: T. gondii tachyzoites (RH virulent strain) were derived from culture cells at the Indonesian &#13;
Research Center for Veterinary Sciences. Genotyping was performed on T. gondii DNA extracted from cell cultured &#13;
tachyzoites using 10 genetic markers of PCR-RFLP, namely, B1#1, B1#2, B1#3, SAG1#1, SAG1#2, P30, BAG1, ROP1, &#13;
GRA1, and GRA7, with digestion using the restriction enzyme DdeI.&#13;
&#13;
Results: The 10 genes were amplified by PCR. Among them, three genetic markers, B1#3, ROP1, and GRA1, were &#13;
genotyped by the PCR-RFLP using restriction enzyme DdeI. Overall, the findings showed that the specific RFLP profile of &#13;
digestion of gene regions by DdeI could be used as a specific marker for the virulent biotype causative of toxoplasmosis. In &#13;
addition, virulent strains of T. gondii can be easily detected by these markers.&#13;
Conclusion: Three pairs of primers (B1#3, ROP1, and GRA1) with DdeI have proven useful for the diagnosis of acute &#13;
toxoplasmosis (virulent strain biotype I). This proposed method is relatively simple, rapid, cheap, and can be performed in &#13;
most laboratories, providing a practical approach for the routine analysis of T. gondii strains.</subfield>
  </datafield>
  <datafield tag="856" ind1=" " ind2=" ">
   <subfield code="a">www.doi.org/10.14202/IJOH.2021.196-203</subfield>
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