DEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA
Data in Indonesia show that around 7 million Indonesians are infected with <br /> <br /> Hepatitis C virus. Therefore the development of a quantitative diagnostic test to <br /> <br /> detect the disease is needed. Until now several commercial assays had been <br /> <...
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id-itb.:213562017-10-02T09:13:02ZDEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA PUTRI NINGSIH (NIM: 21114018), AYU Indonesia Theses INSTITUT TEKNOLOGI BANDUNG https://digilib.itb.ac.id/gdl/view/21356 Data in Indonesia show that around 7 million Indonesians are infected with <br /> <br /> Hepatitis C virus. Therefore the development of a quantitative diagnostic test to <br /> <br /> detect the disease is needed. Until now several commercial assays had been <br /> <br /> developed to quantify the number of virus RNA in a person’s body as well as <br /> <br /> monitor the succes of antiviral therapy. But some of the existing comercial assays <br /> <br /> could not be fully implemented in Indonesia, especially in areas far from the city <br /> <br /> centre, due to their high operational costs. Given the very diverse HCV genome, <br /> <br /> some of these viral infections could not be detected with existing commercial <br /> <br /> assays. Based on this, in this study had developed an alternative test using Real- <br /> <br /> Time PCR method to detect and quantify the viral HCV RNA genotype <br /> <br /> commonly found in Indonesia (subtype 1a, 1b, 1c, 2a, 2e, 2f, 3a, 3k, and 4a) . In <br /> <br /> this study candidate pairs of primers obtained from the NCBI database were <br /> <br /> selected based on the HCV genomic conserved region that amplified the 5’UTR <br /> <br /> HCV fragment with a156 bp amplicon length(base sequence position: 74-229). <br /> <br /> The positive control used was a pUC57 plasmid containing a synthetic gene of <br /> <br /> 5’UTR HCV fragment designed using the Bioedit Sequence Alignment Editor <br /> <br /> software. The sensitivity and linearity of the developed assays determined by <br /> <br /> using the standard plasmid as a positive control. To know about the linearity of <br /> <br /> the standard curve, serial dilution of the positives control is made of <br /> <br /> aconcentration of 1011 copies/mL up to 101 copies/mL. The developed assay had <br /> <br /> linearity at the limit of 1011-106 copies/mL. Efficiency of assay developed was <br /> <br /> 67% with r value = 0,9912. Based on this, this Real-Time PCR method can be <br /> <br /> used as an easy and efficiet alternative diagnostic test to detect and quantify viral <br /> <br /> load of HCV with the lowest quantifiable limit 106 copies/mL. text |
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| description |
Data in Indonesia show that around 7 million Indonesians are infected with <br />
<br />
Hepatitis C virus. Therefore the development of a quantitative diagnostic test to <br />
<br />
detect the disease is needed. Until now several commercial assays had been <br />
<br />
developed to quantify the number of virus RNA in a person’s body as well as <br />
<br />
monitor the succes of antiviral therapy. But some of the existing comercial assays <br />
<br />
could not be fully implemented in Indonesia, especially in areas far from the city <br />
<br />
centre, due to their high operational costs. Given the very diverse HCV genome, <br />
<br />
some of these viral infections could not be detected with existing commercial <br />
<br />
assays. Based on this, in this study had developed an alternative test using Real- <br />
<br />
Time PCR method to detect and quantify the viral HCV RNA genotype <br />
<br />
commonly found in Indonesia (subtype 1a, 1b, 1c, 2a, 2e, 2f, 3a, 3k, and 4a) . In <br />
<br />
this study candidate pairs of primers obtained from the NCBI database were <br />
<br />
selected based on the HCV genomic conserved region that amplified the 5’UTR <br />
<br />
HCV fragment with a156 bp amplicon length(base sequence position: 74-229). <br />
<br />
The positive control used was a pUC57 plasmid containing a synthetic gene of <br />
<br />
5’UTR HCV fragment designed using the Bioedit Sequence Alignment Editor <br />
<br />
software. The sensitivity and linearity of the developed assays determined by <br />
<br />
using the standard plasmid as a positive control. To know about the linearity of <br />
<br />
the standard curve, serial dilution of the positives control is made of <br />
<br />
aconcentration of 1011 copies/mL up to 101 copies/mL. The developed assay had <br />
<br />
linearity at the limit of 1011-106 copies/mL. Efficiency of assay developed was <br />
<br />
67% with r value = 0,9912. Based on this, this Real-Time PCR method can be <br />
<br />
used as an easy and efficiet alternative diagnostic test to detect and quantify viral <br />
<br />
load of HCV with the lowest quantifiable limit 106 copies/mL. |
| format |
Theses |
| author |
PUTRI NINGSIH (NIM: 21114018), AYU |
| spellingShingle |
PUTRI NINGSIH (NIM: 21114018), AYU DEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA |
| author_facet |
PUTRI NINGSIH (NIM: 21114018), AYU |
| author_sort |
PUTRI NINGSIH (NIM: 21114018), AYU |
| title |
DEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA |
| title_short |
DEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA |
| title_full |
DEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA |
| title_fullStr |
DEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA |
| title_full_unstemmed |
DEVELOPMENT OF REAL-TIME PCR METHOD TO DETECT VARIOUS SUBTYPES OF HEPATITIS C VIRUS COMMONLY FOUND IN INDONESIA |
| title_sort |
development of real-time pcr method to detect various subtypes of hepatitis c virus commonly found in indonesia |
| url |
https://digilib.itb.ac.id/gdl/view/21356 |
| _version_ |
1821120437568929792 |