Human Immunodeficiency Virus (HIV) Reverse Transcriptase Activity Correlates with HIV RNA Load: Implications for Resource-Limited Settings

Measurement of human immunodeficiency virus type 1 (HIV-1) plasmaRNA levels using Roche AMPLICOR version 1.5 (HIV RNA) is anintegral part of monitoring HIV-infected patients in industrializedcountries. These assays are currently unaffordable in resource-limitedsettings. We investigated a reverse transcriptase (RT) assayas a less expensive alternative for measuring viral burden thatquantifies RT enzyme activity in clinical plasma samples. Acomparison of RT and HIV RNA assays was performed on 29 pairedplasma samples from patients living in the United States and21 paired plasma samples from patients living in Cameroon. RTlevels correlated significantly with plasma HIV RNA viral loadsin plasma from U.S. patients (r = 0.898; P < 0.001) and Cameroonianpatients, a majority of whom were infected with HIV-1 cladetype CRF02_AG (r = 0.669; P < 0.01). Among 32 samples withHIV viral load of >2,000 copies/ml, 97% had detectable RTactivity. One Cameroon sample had undetectable RNA viral loadbut detectable RT activity of 3 fg/ml. The RT assay is a simpleand less expensive alternative to the HIV RNA assay. Field studiescomparing these assays in resource-limited settings are warrantedto assess the practicality and usefulness of this assay formonitoring HIV-infected patients on antiretroviral therapy.

INTRODUCTION

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Introduction

Human immunodeficiency virus (HIV) plasma viral load measurementis an integral part of monitoring infected patients in industrializedcountries to determine the need to initiate or change antiretroviral(ARV) therapy. A commonly used Food and Drug Administration-approvedassay, the Roche AMPLICOR version 1.5 (HIV RNA), is unaffordablefor most patients in resource-limited settings. This HIV RNAassay uses nucleic acid amplification by PCR of conserved genesequences, including non-clade B sequences (4, 9). One alternativeto measuring RNA copies is to measure the activity of the virus-encodedreverse transcriptase enzyme (RT). An RT assay kit, ExaVir Loadversion 2, is currently available and distributed in Africa,but no published studies to date have correlated version 2 ofthe RT assay with HIV RNA viral load. We describe this correlationin plasma samples from HIV-infected patients from New York andCameroon.

MATERIALS AND METHODS

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Materials and Methods

Plasma samples from HIV-infected patients in New York City and Cameroon. New York City. Twenty-nine anonymous plasma samples from HIV-infected personsattending New York University Medical Center in 2004 were studied.Specimens were presumed to contain predominantly clade B HIV-1virus, although clade analysis was not performed on these samples.While information on clinical symptoms or antiretroviral therapyhistory was not available for this anonymous sample, a largeproportion of patients attending this clinic receive antiretroviraltherapy. All samples were processed within 6 h and stored at–70°C.

Cameroon. Twenty-one anonymous plasma samples from Bamenda, Cameroon,were obtained as part of a larger study (3). All patients wereantiretroviral treatment naïve. Blood was collected inblood bags containing the anticoagulant citrate acid dextrose,which was shipped at room temperature by express courier approximately1 to 3 days after collection (3). Upon arrival, plasma was aliquotedand stored at –70°C. Sequence and phylogenetic analysiswas performed on a subset of the cohort demonstrating that thepredominant clade type was the circulating recombinant form,CRF02_AG (3, 5).

RT assay. RT activity was quantified using the RT activity kit (ExaVirLoad [version 2]; Cavidi Tech-AB, Uppsala, Sweden), as recommendedby the manufacturer (7). One-milliliter plasma samples wereincubated for 1 h at room temperature with a protein-reactivereagent [100 µl of 220 mM 5,5'-dithio-bis(2-nitrobenzoicacid) in 0.8 M Tris, pH 8.1] (7) to destroy cellular polymerasespresent in the plasma while preserving intact RT contained withinvirions. Next, 1.5 ml of an ion-exchange gel (Fractogel EMDTMAE Hicap; in 209 mM morpholineethanesulfonic acid [pH 5.0],275 mM KI, and 0.5 g/liter heparin) (7) was added to each tubeand incubated for 90 min at room temperature on an end-over-endshaker. The gel immobilizes the HIV particle by binding to thelipid membrane of the virion. After thorough mixing, sampleswere transferred to 10-ml plastic filtration columns mountedin a vacuum manifold. Vacuum is applied to isolate the ion-exchangegel particles bound to virions trapped by the filter. The fixedgel was washed four times with 9 ml of wash buffer to removeRT activity-blocking antibodies and antiviral drugs. A furthertwo washes with 9 ml of gel were performed to create a suitableenvironment for RT release after virion lysis. Using 500 µlof lysis buffer, lysates containing RT were collected into individualtest tubes and used directly in the RT activity assay describedbelow.

RT activity was assayed by adding lysates to a 96-well microtiterplate which had a poly(A) nucleotide chain covalently boundto the base of each well. A mix of 5' bromodeoxyuridine triphosphate(BrdUTP) was added, and the plate was incubated at 33°Cfor 48 h.

The plate was washed to terminate the reaction and a BrdU-bindingantibody conjugated to alkaline phosphatase (AP) was added andincubated at 33°C for 90 min.

Following a second wash, the AP substrate p-nitrophenyl phosphatewas added and the resulting yellow color change was measuredto quantify the amount of incorporated BrdUTP. Following additionof the AP substrate each plate was read at three time points:10 min, 2 to 3 h, and 5 to 6 h or overnight at 15 to 24 h. Theresults were expressed in femtograms HIV-1 RT activity/milliliterplasma. The lower limit of detection was <1 fg/ml. Resultswere calculated using ExaVir Load Analyzer software that automaticallydetermines the amount of RT activity in samples using a standardcurve generated from an 11-point dilution of a known amountof recombinant HIV-1 RT. The results are also given in unitsof HIV-1 RNA equivalent copies/milliliter using a conversionfactor derived from a Swedish cohort comprised mainly of subtypeB virus. We report only reverse transcriptase activity in thispaper. Assay precision was determined on duplicates of fivesamples, and assay reproducibility was determined on seven samplesrun on different days.

Plasma HIV RNA assay. HIV RNA load was determined using the ultrasensitive formatof the AMPLICOR HIV-1 Monitor version 1.5 assay (Roche-Diagnostics,Branchburg, N.J.) in identical plasma samples to those usedfor the RT assay. The lower limit of detection was 50 copies/mland the upper limit of detection was 100,000 copies/ml (4).

Statistical analysis. For purposes of analysis, samples with <1 fg/ml of activitywere arbitrarily assigned a value of 0.9 fg/ml, and sampleswith viral load of $≥$ 100,000 copies/ml were arbitrarily assigneda viral load of 100,000 copies/ml. The Spearman rank correlationcoefficient was used to compare results of the two assays. Continuousvariables were analyzed using Student's t test. Correlationof variation was calculated on duplicate samples to determinereproducibility of the RT assay. All statistical analyses wereconducted using SPSS for Windows version 11.0 (SPSS, Inc., Chicago,Ill.).

RESULTS

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Results

Fifty plasma samples from the New York and Cameroon cohortswere tested using both RT and HIV RNA assays (Table 1). Overallconcordance was 76% (38 of 50 samples tested positive in bothassays; no sample tested negative in both assays). A positiveresult in the RT assay alone was found in one sample. Eleven(22%) samples tested positive with the HIV RNA assay alone andhad an HIV viral load below 3,000 copies/ml (median, 326; range,60 to 2,955), and all were from the New York cohort. Among 32samples from either cohort with an HIV viral load of >2,000copies/ml, 3% had undetectable RT activity whereas among 18samples with a viral load of $≤$ 2,000 copies/ml, 56% had undetectableRT activity. A strong correlation was found between RT activityand HIV RNA viral load among all clade B and non-clade B samples(r = 0.869; P < 0.01) (Figure 1).

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TABLE 1. HIV-1 RNA viral load by PCR and reverse transcriptase (RT) activity for Cameroon and New York City

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FIG. 1. Correlation of HIV load based on RT activity and HIV RNA assay (log₁₀ values). Cameroon and New York City cohorts (n = 50). The lower limit of detection were 1.7 log₁₀ RNA copies/ml (50 copies/ml) and –0.05 log₁₀ RT activity/ml (0.9 fg/ml). The upper limit of detection for the HIV RNA assay was 5 log₁₀ RNA copies/ml (100,000 copies/ml), and samples above this detection limit were attributed arbitrary values of 5 log₁₀ RNA copies/ml. All data are shown and included in the correlation; r, Spearman correlation coefficient.

New York City cohort. Eighteen (62%) of the 29 plasma samples from the New York Citycohort tested positive for both RT activity and HIV RNA. Themedian HIV RNA viral load was 2,067 copies/ml (range, 60 to>100,000 copies/ml); the median RT activity was 10 fg/ml(range, <1 to 2,400 fg/ml). Among samples with HIV RNA PCRlevels of $≥$ 50 and $≤$ 3,000 copies/ml, 11 (69%) had undetectableRT activity. Among the 13 samples with HIV RNA PCR levels of>3,000 copies/ml, all had detectable RT activity. A strongcorrelation was found between RT activity and HIV RNA viralload in the New York cohort (r = 0.898; P < 0.01).

Cameroon cohort. Twenty of the 21 samples from the Cameroon cohort tested positiveusing both RT and HIV RNA assays. The one discordant samplehad undetectable viremia (<50 copies/ml) and detectable RTactivity (3 fg/ml). Overall, the median viral load in this cohortwas 21,831 copies/ml (range, <50 to >100,000 copies/ml),and the median RT activity was 32 fg/ml (1 to 536 fg/ml). Asignificant correlation was found between RT activity and HIVRNA viral load among the HIV-1 non-clade B samples (r = 0.669;P < 0.001).

Duplicates of five Cameroon samples were assayed in the samerun and had a mean of 1.87 fg/ml with a coefficient of variationof 7.9%. Duplicates of six Cameroon samples were assayed intwo different runs and had a mean of 1.60 fg/ml with a coefficientof variation of 8.6%.

DISCUSSION

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Discussion

This is the first study to evaluate version 2 of the RT assayin clade B or non-clade B plasma samples. We found a significantcorrelation between the RT and HIV RNA assays in estimatingviral load in patient plasma samples from New York City andCameroon. The correlation between the two assays was strongin the New York cohort, consistent with findings of previousstudies conducted in persons infected with clade B virus (8)and moderate but significant in the non-clade B cohort. Thenumber of samples in the New York cohort with RNA viral loadsof <2,000 copies is striking. The most likely explanationfor this observation is that the majority of patients in theNew York cohort were receiving antiretroviral treatment, althoughthe specific proportion of treated patients was unknown.

The weaker correlation between RT activity and HIV RNA viralload in the Cameroon cohort may be a result of several factors.Most significantly, the long transport time of the Cameroonsamples may have affected the RT and the RNA PCR assays to differentdegrees, therefore adversely affecting their correlation. Itis noteworthy that although the manufacturer of the RT assayrecommends that all blood samples be processed within 6 h ofacquisition and frozen at –20°C before analysis, infact, the RT assay performed well and correlated closely withHIV RNA viral loads despite the delay between blood draw andprocessing. This suggests that the RT assay is robust and maybe useful in the field setting where collection and processingtime may vary. Another possibility for the weaker correlationin the Cameroon cohort is that the sensitivity of the second-generationHIV RNA assay may be reduced for recombinant HIV genomes suchas those frequently found in Cameroon. Of note, however, oneprevious study evaluating three viral load methods for detectingcirculating recombinant strains such as AG found Amplicor version1.5 to be accurate and reliable (1).

Published studies evaluating the ExaVir Load RT assay are few,and none have evaluated version 2 (2, 7). Braun et al. comparedthe RT assay, version 1, with RNA PCR in 322 plasma samplesincluding 66 non-clade B subtypes (2). A strong correlationwas found between the two assay (r = 0.850; P < 0.0001) independentof subtype. The sensitivity of the RT assay, version 1, waspoor for samples with viral load of 10,000 copies/ml or below(2). Malmsten et al. compared the RT assay, version 1, to RNAPCR (Roche Amplicor version 1.5) in 390 plasma samples frompatients living in Sweden (7). The correlation was strong (r= 0.90, P < 0.0001); however, RT activity was detectablein only 50% of samples with a viral load between 2,500 and 6,900copies/ml (2). The RT assay was also evaluated by the manufacturerand researchers in Uganda in a cohort of patients from Uganda(8). This study compared the RT assay, version 1, and RNA viralload in a cohort of 46 patients from Uganda, and they reportthat while correlation was good (R² = 0.85) overall, RT activitywas detected in only 47% of samples with a viral load of lessthan 55,000 copies/ml (8).

Improvements have been made to the first version of the ExaVirLoad RT assay to increase sensitivity. These changes includedimproved wash of the gels containing immobilized virions, improvedvirion lysis to increase the RT enzyme yield, use of largerlysate volume, and a longer RT reaction time (approximately40 h) (6). The manufacturer reports that in 262 clinical samples,the detection limit of version 2 of the ExaVir RT assay was400 RNA copies/ml, below which only 19% of 52 samples had detectableRT activity. However, among 93 samples containing 51 to 1,500RNA copies/ml, only 39 (42%) had detectable RT activity (6).Similarly, our study found 6 (40%) of 15 samples containing50 to 1,500 RNA copies/ml had detectable RT activity but that31 (97%) of 32 samples containing >2,000 copies/ml had detectableRT activity. Therefore, the detection limit of the RT assayin our study is approximately 2,000 copies/ml, higher than thatreported by the manufacturer (6).

Low cost and technical simplicity are two advantages of theRT assay. The setup for the RT assay includes the ExaVir Loadstart-up kit ($3,000 U.S.) and the assay kit itself. The start-upkit includes a sample box and lid, column holder, waste collector,sample collector, tube rack, vacuum pump, waste container, bufferdispenser, 4 3-liter wash buckets, various plastic bottles andracks, and ExaVir Load Analyzer software. Other equipment thatis required but not provided include an enzyme-linked immunosorbentassay reader, an end-to-end mixing table, an incubator, pipettes(including multichannel pipettes), and a –20°C refrigerator.Each ExaVir Load kit contains reagents and consumables for analysisof 28 samples, one negative control, and one positive control.Disadvantages of this assay include the requirement for 1 mlof plasma (of particular concern for pediatric patients), lackof standard positive and negative controls in the kit, and theneed for 3 days to complete the assay. The cost per ExaVir Loadkit currently is approximately $843.75 U.S. when purchased fromlocal Kenyan distributors, which is approximately $28.13 pertest, not including start-up costs and technician time. Whileconsiderably less expensive than the HIV RNA assay, which isapproximately $100 U.S. per test when performed in Kenya, currentlythe RT assay may be too costly to recommend for routine usein resource-limited settings.

Measurements taken by HIV RNA PCR and RT assays represent differentaspects of viral replication. Plasma HIV RNA assays measurevirion-associated RNA while the RT assay measures the activityof a virion-associated enzyme required for replication. Measuringenzyme activity as marker for viral replication has severaladvantages in the international setting aside from cost. Thereverse transcriptase enzyme is well conserved across differentgenetic clade types, therefore the RT assay would be expectedto function well in areas of the world where non-clade B strains,including complex recombinant strains, are common. Our datasuggest that the RT assay is able to detect RT activity in plasmacontaining complex recombinant non-B subtype HIV virus. In addition,RNA-based methods do not differentiate between functional anddefective virions and therefore may not reflect true viral replicationactivity, whereas the RT assay quantifies actual reverse transcriptaseactivity.

In the search for more affordable alternatives for viral loadmeasurement for monitoring of HIV-1-infected patients livingin resource-limited settings, the RT assay appears promising.RT assay results for both U.S. and Cameroon cohorts correlatewell with the HIV RNA assay and demonstrate adequate sensitivityabove 2,000 copies/ml. However, the usefulness of the RT assayin monitoring patients on antiretroviral therapy in a resource-limitedsetting is unknown. Field trials of the RT assay in such settingswill be important to assess the cost, ease, and applicabilityof this assay in routine HIV care.

ACKNOWLEDGMENTS

We thank Paul Nickolopalous for assistance with the Roche Amplicorassay; Maura Laverty for administrative support; Gary Corriganfrom Cavidi-Tech for technical support; Sherri Burda and ConstanceWilliams for processing of the Cameroon specimens; Charles Gonzalezfor assistance in obtaining plasma samples from the New YorkCity cohort; Steven Oliver for laboratory assistance; and JoelErnst and Judith Aberg for their critical reading of the manuscript.

New York University Centers for AIDS Research DiscretionaryFunds was the source of funding.

FOOTNOTES

* Corresponding author. Mailing address: 550 First Avenue, C&D Building, 5th Floor, New York University Medical Center, Division of Infectious Disease, New York, NY 10016. Phone: (212) 263-0766. Fax: (212) 263-8264. E-mail: sumathi.sivapalasingam{at}med.nyu.edu.

REFERENCES

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