Patients failing antiretroviral treatment for extended periods of time are at risk of accumulating HIV drug resistance mutations (DRMs), which negatively influences second-line treatment. This ...retrospective study assessed the rate of DRM accumulation among South African patients with continued virological failure. Serial genotypic resistance testing was performed and DRMs were scored according to the 2009 IAS-USA list. Among 43 patients, 38 (88.4%) harbored ≥1 DRM. The median time between two sequential resistance tests was 5 months (IQR: 3-10). Thymidine analogue mutations accumulated at a rate of 0.07 mutation per month of drug exposure, which is faster than previously reported. Routine virological monitoring should be implemented in resource-limited settings to preserve susceptibility to second-line regimens.
A dissertation submitted to the Faculty of Health Sciences, University of the Witwatersrand , in fulfillment of the requirements for the degree of Master of Science in Medicine, 2013
Sequence ...analysis from HIV-1 (human immunodeficiency virus type 1) subtype B and more;
recently subtype C infected patients has revealed that mutations in the HIV-1 protease region;
that confer drug resistance to boosted protease inhibitor (PIs) are rarely detected at the time;
of virological failure. Mutations in the HIV-1 subtype B gag-pol cleavage sites are thought to;
be compensatory mutations which arise as a result of PI use. This study investigated the;
presence of compensatory mutations in the HIV-1 subtype C gag-pol cleavage sites and;
matched pol genotypes from South African patients failing a boosted PI-based regimen, as;
compared to antiretroviral drug naïve patients.;
A new amplification protocol encompassing the near full-length gag, PR and partial RT was;
established and used to sequence the HIV-1 gag-pol cleavage sites from 23 proviral DNA;
samples (p24 antigen cultured peripheral blood mononuclear cells; PBMCs), and 51 patient;
samples (23 antiretroviral drug-naïve, 26 failing second-line lopinavir/ritonavir containing;
regimens), all attending the Charlotte Maxeke Johannesburg Hospital. Nucleotide sequences;
were aligned and codon positions S373Q, A431V, I437T/V, L449P or P453L associated with;
known gag-pol cleavage site mutations were analysed and compared. The pol genotypes were;
established using an in house assay. Antiretroviral drug resistant primary virus isolates were;
grown from samples from patients enrolled on the CIPRA-SA study, and propagated in coculture;
with PHA-activated, IL-2 stimulated PBMCs. HIV-1 gag-pol cleavage sites and pol;
genotypes for all primary virus isolates were established as described above.;
Fifty one of 74 patient samples, used to establish the in-house gag-pol cleavage site assay,;
were successfully amplified and sequenced. Detailed analysis of the five known gag-pol;
cleavage sites revealed that 5 patient samples (4 PI-exposed, 1 unknown regimen) encoded;
for the previously described mutations that impact on gag-pol cleavage in the absence of any;
major PR mutations. A further five samples from patients on the failing PI-based regimen had;
major PR mutations. No known mutations in the gag-pol region were identified in patients;
failing a first line regimen. The pol mutations described in this study were similar to the;
findings reported for treatment failures in South African HIV-1 subtype C infected patients.;
Primary virus was grown from only 25 of the 91 PBMC CIPRA samples. None of the 25;
CIPRA-SA primary virus isolates had gag-pol cleavage site mutations, and only 9 harboured;
known RT antiretroviral drug resistant mutations.;
Overall, the presence of HIV-1 gag-pol cleavage site mutations may account for virological;
treatment failure in 5 of the South African patient samples analysed. Although the gag-pol;
cleavage site mutations detected in the current study are only present in a small proportion of;
treatment-experienced South African patients, this may increase due to more patients;
accessing second line PI-containing regimens. Thus, future genotyping work incorporating;
the analysis of the gag-pol cleavage sites in addition to the PR and RT regions is warranted.;
The antiretroviral drug resistant primary viruses obtained provide valuable reagents for future;
phenotyping studies.