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Journal of Clinical Microbiology, January 1998, p. 258-260, Vol. 36, No. 1
Department of Microbiology and Immunology,
University of North Carolina at Chapel Hill, Chapel Hill, North
Carolina1;
New England Research
Institute, Watertown, Massachusetts2;
and
Organon Teknika, Durham, North
Carolina3
Received 30 May 1997/Returned for modification 30 July
1997/Accepted 1 October 1997
We compared whole blood dried on filter paper to the standard assay
with frozen cell-free plasma for use in the quantitation of the human
immunodeficiency virus RNA load in blood. RNA values from filter paper,
corrected for the hematocrit, gave results comparable to those of the
standard assay in terms of sensitivity and reproducibility.
The measurement of human
immunodeficiency virus (HIV) RNA levels in plasma is rapidly becoming
the most important laboratory tool for staging HIV infection and for
the management of therapy (6, 7). However, quantitation of
HIV levels in plasma requires access to certain laboratory equipment
which may not be readily available in some settings. By the year 2000 the World Health Organization predicts that 30 million to 40 million
new HIV infections will have occurred, with 90% of these occurring in
developing countries (5). Even the simple act of
centrifuging a tube of blood, aliquoting and freezing the plasma, and
subsequently shipping the plasma to a centralized laboratory might
prove difficult in some field situations, where many clinical trials of
new antiretroviral drugs and potential HIV vaccines as well as
transmission intervention studies will be conducted in the future.
The purpose of this research was to develop a simple method for
collecting specimens for analysis of the HIV RNA level in plasma that
would yield accurate and reproducible results without the need for
electricity at the collection site. Our ultimate goal is to obtain
blood from a fingerstick or heelstick, dry it on filter paper, and
airmail it to a central laboratory, thus avoiding the need for a
skilled phlebotomist and laboratory technician on site and also
avoiding the need for centrifuges, freezers, and dry ice for shipping.
Dried blood spots have been used for many years to screen for several
metabolic disorders such as phenylketonuria and sickle cell disease.
For HIV they have been used for the anonymous screening of newborns to
assess the seroprevalence of HIV among childbearing women
(4) and for the diagnosis of perinatal HIV infections by
using HIV DNA (2, 3). More recently, it has been reported
that DNA obtained from dried blood spots is suitable for gene sequence
analysis (1). Consequently, we decided to evaluate the
possibility of using whole blood dried onto filter paper for the
quantitation of the HIV RNA level in plasma.
One hundred four HIV-positive patients seen in the University of North
Carolina's adult and pediatric infectious disease clinics provided 4 ml of blood collected in EDTA for the purposes of viral load testing.
HIV RNA was quantitated from 100 µl of whole blood from each of 76 patients spotted in quadruplicate onto Schleicher & Schuell no. 903 filter paper. A total of 50 µl of whole blood from an additional 28 patients was spotted in eight replicates onto Schleicher & Schuell
Isocode filter paper. The blood spots were dried overnight at room
temperature in a biohazard hood. We also used the whole blood to
determine the hematocrit (mean of two determinations). Cell-free plasma
obtained from the same tube of blood was stored at We initially used the no. 903 paper to measure HIV-1 RNA levels from
dried blood spots, with encouraging results (Fig.
1A). However, a second lot of paper gave
uninterpretable results and we switched to Isocode paper, which is
pretreated with guanidinium isothiocyanate. The log10
hematocrit-corrected RNA concentration from the two types of paper is
compared with the log10 RNA concentration from plasma in
Fig. 1A (no. 903 filter paper) and Fig. 1B (Isocode filter paper). The
diagonal line on each graph indicates where the points would fall if
the estimates from the dots and the plasma were the same. Correlation
coefficients were 0.88 (no. 903 filter paper versus plasma) and 0.90 (Isocode filter paper versus plasma). There is little evidence of a
systematic difference between the values from no. 903 filter paper and
those from plasma. The mean difference, 0.0478, was not statistically
significantly different from zero (P = 0.33). Most
(91%) of the differences in RNA values between the no. 903 filter
paper dots and plasma were between
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Copyright © 1998, American Society for Microbiology. All rights reserved.
Quantitation of Human Immunodeficiency Virus Type 1 RNA in Plasma by Using Blood Dried on Filter Paper
ABSTRACT
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70°C. HIV type 1 (HIV-1) RNA levels were determined by a commercially available nucleic
acid sequence-based amplification assay (NASBA; NASBA HIV-1 QT; Organon
Teknika, Durham, N.C.). Two 50-µl aliquots of dried blood spots were
placed in 9 ml of NASBA lysis buffer, and the mixture was rocked at
room temperature for 2 h to isolate the RNA, after which the
filter papers were removed. The HIV-1 RNA from cell-free plasma was
isolated by placing 100 µl of plasma in 0.9 ml of NASBA lysis buffer.
For the rest of the procedure, the manufacturer's instructions were followed, including the use of diluted calibrators. The numbers of RNA
copies per milliliter of plasma from the spots were calculated as
follows: corrected number of spot RNA copies per milliliter of
plasma = (number of spot RNA copies per milliliter of
blood)/[(100 hematocrit)/100]. Blood from the first 76 patients was tested singly by using the no. 903 filter paper. Blood
from the remaining 28 patients was tested in duplicate by using the
Isocode filter paper. Some dried spots were stored at room temperature
for various lengths of time before testing.
0.5 and 0.5 log10.
However, the mean difference between values from plasma and Isocode
filter paper was significantly different from zero (mean = 0.22;
P < 0.01). On average, then, the values from plasma
were 1.66 times the values from the Isocode filter paper. The
difference did not vary systematically over the range of the data (Fig.
1B), so the use of a correction factor for the Isocode paper might be
feasible.
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FIG. 1.
(A) Log10 hematocrit-corrected HIV RNA
concentrations for 55 patients tested with no. 903 filter paper plotted
against the log10 RNA concentration for the matching plasma
sample. Samples for which either estimate was below the detection
limits were excluded (n = 21). The diagonal line
indicates where points would fall if the estimates from the dots and
the plasma were the same (correlation coefficient = 0.88). The
points in the plot are roughly scattered around this line, indicating
that there is little evidence of a systematic difference between the
two approaches. For 91% of the hematocrit-corrected dot values, the
values were within threefold (0.5 log10) of the value for
plasma. (B) Mean log10 hematocrit-corrected HIV RNA
concentrations for the Isocode filter paper plotted against the mean
log10 RNA concentration for the matching plasma sample
(coefficient correlation = 0.90). The points are shifted to the
right, indicating that higher values were obtained in the assay with
plasma. The mean difference was 0.22 (P = 0.0016),
meaning that, on average, the estimates from the plasma were 1.66 times
the estimates from the Isocode filter paper. For 95% of the
hematocrit-corrected dot values, the values were within threefold (0.5 log10) of the value for plasma.
We tried to correct RNA values from filter paper for the hematocrit in three ways. Initially, we simply adjusted the RNA value obtained from the filter paper for each patient's hematocrit, producing the data shown in Fig. 1. Then we tried the use of two constant correction factors. The first, 1.82, was derived from the mean hematocrit of 45 for this cohort. The second, 2.0, was based on the assumption that the mean hematocrit was close to 50. Use of a constant factor could be appropriate when hematocrits are not available. The two constants produced very similar results (data not shown).
The sensitivities of filter dot RNA and plasma RNA were compared by classifying each RNA determination as above or below the limit of detection (1,000 HIV RNA copies/ml). For 21 of 76 (28%) samples, values from no. 903 filter paper were below the detection limit, whereas for 17 of 76 (22%) samples, values from plasma were below the detection limit. For 13 samples, values from both no. 903 filter paper and plasma were below the detection limits. For 9 of 28 (32%) samples at least one of two values was below the detection limit on the Isocode filter paper, whereas for 7 (25%) samples at least one of two values from plasma were below the detection limit. For six samples two values from both Isocode filter paper and plasma were below the detection limits. The sensitivities of assays with filter dot RNA and plasma RNA were not significantly different (P > 0.05), but these results should be interpreted with caution. The volume of plasma on the filter paper dots is roughly half the volume in the plasma assay, so a difference in sensitivity should be expected. The absence of such a difference could simply mean that the study included few patients with RNA concentrations in the range needed to show a difference. Alternatively, it may reflect the fact that the HIV-1 RNA from the dried blood spots included both cell-free and cell-associated HIV-1 RNA, while the HIV-1 RNA quantitated from plasma is essentially only cell-free RNA.
The reproducibility of RNA values was examined by using intra-assay standard deviations (SDs) that were estimated from the duplicate day 0 results for 17 patients from both Isocode paper and plasma. The SDs for Isocode filter paper and plasma were 0.19 and 0.15, respectively. However, one pair of Isocode filter paper values differed by almost 0.7 log10. This large difference may reflect a specimen handling error rather than a problem with reproducibility. When this point is excluded, the SD drops to 0.17, which is close to the SD for plasma. For comparison, in a multicenter evaluation of quantitative assays of HIV-1 RNA levels in plasma, the AIDS Clinical Trials Group virology laboratories determined that the intra-assay SD for NASBA was 0.15 (8).
The stability of estimates from Isocode filter paper was examined by using a random effects regression of the log10 RNA level on length of storage (in days). The results for blood from 14 patients, each with storage times of 0, 7, and 28 days, were included. Nine values that were less than the detection limits were set equal to 3.0 (1,000 HIV RNA copies/ml). A statistically significant decline of 0.0261 log10 RNA copies per day was detected (P < 0.01). This slope is equivalent to a loss of approximately 5% per day.
Initial results for the no. 903 filter paper looked very good. However, later results with a different lot of no. 903 filter paper were not reproducible. It may be that this paper should be handled with gloved hands at all stages, including prior to the application of blood, to avoid contamination with RNases present on fingers; this may not be possible in all situations. The Isocode paper is pretreated with guanidinium isothiocyanate, so it does not require special handling prior to application of the specimen.
The preliminary results reported here are extremely encouraging. Using the Isocode filter paper and correcting for hematocrit and even without correcting for the use of the Isocode filter paper, we were able to quantify the amount of HIV RNA in plasma fairly accurately (Fig. 1B). No difference in sensitivity was observed between the assays with Isocode filter paper and the plasma. The reproducibility of the results of assays with Isocode filter paper were comparable to the reproducibility of the results of the standard assay with plasma. However, problems with stability exist. We are not sure whether the RNA is being degraded with time or whether we are simply having increased difficulty in removing the RNA from the filter paper with prolonged storage.
We believe that modifications and refinements of this method can provide an accurate measurement of the plasma HIV RNA level suitable for primitive field conditions. In addition, the nucleic acid recovered from the spots should be amenable to amplification and sequencing and should thus be of value for drug sensitivity and HIV clade testing (1).
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ACKNOWLEDGMENTS |
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This study was supported in part by cooperative agreements U01-AI27535 and U01 AI38858 (contract 96VD006) from the National Institute of Allergy and Infectious Diseases.
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FOOTNOTES |
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* Corresponding author. Mailing address: University of North Carolina at Chapel Hill, CB# 7140, Chapel Hill, NC 27599-7140. Phone: (919) 966-6872. Fax: (919) 966-9873. E-mail: sfiscus{at}email.unc.edu.
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Journal of Clinical Microbiology, January 1998, p. 258-260, Vol. 36, No. 1
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
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