IDENTIFICATION OF MPT64 GENE MUTATION IN THE CLINICAL ISOLATES OF MYCOBACTERIUM TUBERCULOSIS COMPLEX (MTBC) BASED ON CORD FACTOR DETECTION
Mycobacterium tuberculosis complex (MTBc) infection may have a similar clinical symptom to non-tuberculosis mycobacteria (NTM) infection, but the treatments for these two diseases are very different. Recently, the incidence and prevalence of both Tuberculosis and NTM infection has increased. Thus...
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| Format: | Theses |
| Language: | Indonesia |
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| Online Access: | https://digilib.itb.ac.id/gdl/view/57548 |
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| Institution: | Institut Teknologi Bandung |
| Language: | Indonesia |
| Summary: | Mycobacterium tuberculosis complex (MTBc) infection may have a similar clinical
symptom to non-tuberculosis mycobacteria (NTM) infection, but the treatments for
these two diseases are very different. Recently, the incidence and prevalence of both
Tuberculosis and NTM infection has increased. Thus an accurate differentiation of
MTBc and NTM is needed. The MPT64 Rapid Test is one of the most widely used
MTBc detection methods because it is high in sensitivity and specificity. However,
several studies have reported variations in the accuracy of this test due to potential
mutations in the mpt64 gene. Therefore, all MPT64 test-negative results will be
considered as NTM, potentially leading to misdiagnosis and inappropriate patient
treatment. In addition to MPT64 test, cord factor formation can also be used to
differentiate MTBc from NTM. This study aims to identify and characterize mpt64
gene mutations in the clinical isolates of MTBc from patients with suspected MTBc
infection in Bandung based on the presence of cord factor. MPT64 test (Rapid Test
SD Bioline TBAgMPT64) and cord factor detection were carried out on 1424
mycobacterial isolates. Isolates with MPT64 test-negative but produce cord factor
were then subjected to DNA extraction and PCR amplification using specific primer
for mpt64. Isolates that yielded PCR product were subjected to full-length mpt64
gene sequencing and then analyzed using MUSCLE. The protein structure of mpt64
was predicted using Swiss Model. We found 13 isolates to be MPT64 test-negative
but produce cord factor. Only 7 out of 13 isolates yielded PCR product and
confirmed as MTBc. Sequence analysis of mpt64 showed several mutations which
are 5-bp (1 isolate), 6-bp (1 isolate) and 63-bp deletion (5 isolates). These
mutations are causing amino acid and epitope alteration of mpt64 antigen, causing
them to go undetected by the MPT64 test. Our findings suggest that the presence of
cord factor in MTBc isolate with a negative MPT64 test result may indicate
mutation in mpt64 gene. |
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