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Previous Article | Next Article 
Journal of Clinical Microbiology, April 1998, p. 1008-1014, Vol. 36, No. 4
Institut für Medizinische Mikrobiologie
and Immunologie,1
Urologische
Klinik,2 and
Abteilung für
Transfusionsmedizin,3
Universitäts-Krankenhaus Eppendorf, Hamburg, Germany
Received 2 July 1997/Returned for modification 15 October
1997/Accepted 6 January 1998
The feasibility of the major peripheral blood leukocyte (PBL)
subsets for use in qualitative and quantitative PCR to monitor secondary cytomegalovirus (CMV) infection and ganciclovir therapy was
assessed with 188 blood samples derived from 40 CMV immunoglobulin G-positive renal-allograft recipients. In pp65 antigen-positive patients all leukocyte fractions, but only 79.5% of plasma
preparations, were PCR positive. In pp65 antigen-negative samples from
patients after antiviral treatment only 7.3% of polymorphonuclear cell (PMNL) samples, but 81.8% of peripheral blood mononuclear cells (PBMC), and 10.9% of plasma samples remained PCR positive. Similarly, in patients with latent infections only 5.0% of PMNL, but 51.7% of
PBMC preparations, and 8.0% of plasma samples were PCR positive. Regarding patients with active CMV infection, CMV DNA copy numbers in
PMNL correlated significantly with pp65 antigen-positive cell counts
before and after onset of ganciclovir therapy. Significant differences
in CMV DNA copy numbers in PMNL and plasma were observed (i) between
patients with symptomatic infection and those with asymptomatic
infection and (ii) between patients with active infection and those
with latent infection. In contrast, PBMC harbored equally low CMV DNA
levels both in patients with active infection and those with latent
infections, and no decline of CMV DNA load in PBMC was observed during
antiviral treatment. We conclude that detection of CMV DNA in PMNL, not
in PBMC, is associated with active infections and is more sensitive
than detection of CMV DNA in plasma. Negative PCR results for PMNL
after antiviral therapy indicate recovery, and fewer unwanted
positive results occur compared to PBMC and plasma. Therefore, purified
PMNL should be preferred for analysis by qualitative CMV PCR to avoid
unwanted positive results. The CMV DNA load in PBMC compared with that
in PMNL is negligible during active infection, so mixed PBL are
sufficient for use in quantitative PCR.
The level of viremia plays an
important role in the course of cytomegalovirus (CMV) infection. The
pp65 antigenemia assay and PCR methods for detection of CMV DNA in
peripheral blood leukocytes (PBL) and plasma have been increasingly
utilized in recent years for the rapid diagnosis of active CMV
infection in immunocompromised hosts and for monitoring antiviral
treatment (for reviews, see references 29 and
36). However, the identification of patients at risk
for clinically relevant disease is problematic for various reasons.
Firstly, low-level antigenemia is not necessarily indicative of
symptomatic infections (36). On the other hand, positive PCR
results from leukocytes are often obtained in pp65 antigen-negative samples of patients after successful antiviral therapy and even in CMV
immunoglobulin G (IgG)-positive immunosuppressed individuals with
latent infection (1, 2, 6, 20, 40, 42), although CMV DNA is
only occasionally detectable in healthy seropositive blood donors
(33-35). Plasma has been shown to yield fewer unwanted positive PCR results than PBL (10), but the lower
sensitivity might be problematic with respect to early detection of CMV
relapse or therapy monitoring (9, 10).
To overcome these problems, protocols for quantitative assessment of
antigenemia and DNAemia have been devised, which are now successfully
used for predicting symptomatic infection and for monitoring antiviral
therapy (29). However, the antigenemia assay is error-prone
due to rapid decline of pp65 antigens in blood samples processed with
delay, whereas CMV DNA copy numbers in PBL remain at constant levels
for at least 72 h (30). On the other hand, quantitative
PCR requires elaborate techniques which limit its routine use. Thus,
from the diagnostic standpoint it remains desirable to improve the
clinical utility of qualitative CMV PCR. As PCR with PBL is the most
sensitive, the selective detection of CMV DNA associated with active
infection in PBL would be highly interesting.
Reports on the mechanisms of interaction between CMV and circulating
leukocytes are still controversial (5, 12, 14, 17, 19, 22, 25, 26,
37, 39). Polymorphonuclear leukocytes (PMNL) are the predominant
carriers of pp65 antigen and also harbor CMV DNA during active
infections (5, 12, 15-17, 27). A positive correlation has
been demonstrated between pp65 antigen-positive cell counts and the
overall amount of CMV DNA present in mixed PBL during active infection
(23, 38). However, only little information exists regarding
the quantitative distribution of CMV DNA among leukocyte subpopulations
(3, 27). The exact tropism and state of CMV genomes found in
pp65-negative patients after successful antiviral therapy and in
latently infected immunosuppressed patients are still poorly defined.
CMV DNA occasionally detected in seropositive healthy blood donors is
probably due to persistent viral genomes in peripheral blood
mononuclear cells (PBMC) (33-35).
If the detection of CMV genomes in different leukocyte subsets reflects
different states of the virus, the fraction chosen for PCR analysis
should strongly influence the value of PCR in discriminating between
active and latent CMV infection or in monitoring antiviral therapy.
Therefore, we have compared qualitative and quantitative CMV PCRs for
the major leukocyte subpopulations with plasma PCR for 40 CMV
IgG-positive renal-allograft recipients (i) with active CMV infections
before, during, and after ganciclovir treatment and (ii) with latent
CMV infections.
Patients.
One hundred eighty-eight blood samples from 40 CMV
IgG-positive renal-allograft recipients were analyzed. Only patients
without current antiviral treatment at the time of the first
investigation were enrolled in the study. Patients without evidence of
active CMV infection who were prophylactically treated with ganciclovir during steroid-resistant graft rejection therapy (anti-lymphocyte globulin [ATG] and/or OKT3) were excluded as well. Samples were collected weekly during the primary hospitalization phase (between 21 and 50 days after transplantation). Patients treated with ganciclovir during primary hospitalization were monitored every other day for 2 weeks and at weekly intervals for up to 5 further weeks. From five
patients samples were drawn every 2 days for 2 weeks upon readmission
to the ward due to active CMV infections between days 90 and 160 posttransplantation. All samples were analyzed prospectively.
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Utility of Major Leukocyte Subpopulations for Monitoring
Secondary Cytomegalovirus Infections in Renal-Allograft Recipients
by PCR
ABSTRACT
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
Isolation of leukocytes. Ten milliliters of whole blood was collected in EDTA tubes and processed within 4 h postdrawing. Mixed PBL were isolated by centrifugation of 2 ml of whole blood at 700 × g for 3 min and subsequent lysis of erythrocytes with 0.8% ammonium chloride. Pelleted PBL were washed with phosphate-buffered saline, pH 7.4, and quantitated with a hematological cell counter. The proportions of PMNL and PBMC were determined, and aliquots containing 105 cells were subjected to antigenemia assay and PCR, respectively.
PBMC (lymphocytes and monocytes) and PMNL were semipurified by Ficoll-metrizoate density centrifugation using Lymphoprep and Polymorphprep (Nycomed, Oslo, Norway) according to the manufacturer's instructions and quantitated. PBMC fractions contained about 5% PMNL, and PMNL fractions were contaminated by 5% lymphocytes and monocytes on average as determined by Giemsa staining and morphological analysis. Subfractions were adjusted with phosphate-buffered saline to the number of PMNL and PBMC per milliliter determined in 106 mixed PBL.Antigenemia assay.
A total of 105 mixed PBL (100 µl) were centrifuged onto glass slides, fixed, and permeabilized with
5% paraformaldehyde-0.5% Nonidet P-40, and pp65 antigen was detected
in PMNL by indirect immunofluorescence as described previously
(11) using Clonab CMV (Biotest, Dreieich, Germany) by
following the manufacturer's instructions. Results were expressed as
the average of two pp65-positive cell counts with deviations 
20% for
cell counts 
100 and deviations 30% for counts 50 (data not
shown).
DNA extraction from leukocytes and plasma. DNA was extracted from 500 µl of mixed PBL, PMNL, and PBMC preparations (equivalent to the number of cells present in 5 × 105 mixed PBL) by digestion with 100 µg of proteinase K (8, 28) per ml in a 50-µl reaction volume. After being boiled for 10 min, a 10-µl supernatant sample was subjected to PCR.
Plasma was obtained by centrifugation of 1 ml of whole blood at 700 × g for 10 min to remove cells. Supernatants (approximately 500 µl) were centrifuged for a second time to remove cell debris and then extracted once with 1 volume of phenol-chloroform and subsequently with 1 volume of chloroform-isoamyl alcohol (24:1). DNA from 100 µl of the aqueous phase was precipitated with 0.1 volume of sodium acetate, pH 5.2, and 2.5 volumes of absolute ethanol. After centrifugation at 15,000 × g for 30 min, pellets were washed with 70% ethanol and resuspended in 100 µl of H2O. A 10-µl sample was subjected to PCR.CMV PCR.
CMV and 
-globin target sequences were
quantitated by competitive PCR using cloned standard (ST) sequences as
described elsewhere (20, 28) with slight modifications. The
CMV ST sequence was generated in PCR by site-directed mutagenesis and
subcloned into the vector pSPT19 (Boehringer Mannheim, Mannheim,
Germany) (20). It contained three successive point mutations
compared to the amplified coding region of glycoprotein B derived from
the CMV laboratory strain AD169 (4). The cloning of the
-globin ST was previously described (18).
-globin ST and either 103 copies (high ST) or 50 copies
(low ST) of the CMV ST. CMV target sequences were amplified in 20 cycles with the external CMV-specific primers E1
(5'-TCCAACACCCACTAGACCGGT-3') and E2
(5'-CGGAAACGATGGTGTAGTTGG-3') (8). Ten
microliters each of the external reaction mixture was reamplified in a
second round of PCR for 30 cycles with the internal CMV-specific
primers TGGE1B
(5'-CCGGATCCCGCCGCCCGCCCCGCGCCCGCCGCGGCAGCACCTGGCT-3') and
TGGE2E (5'-GCGAATTCGTAAACCACATCACCGTGGA-3') and the
-globin-specific primers 1aB
(5'-CCGGATCCCGCCGCCCGCCCCGCGCCCCTGCCGTTACTGCCCTGT-3') and
1bE (5'-GCGAATCCTATTGGTCTCCTTAAACCTG-3'), respectively. ST and wild-type CMV and -globin PCR amplimers were quantitated by
hybridization to a strand-specifically labeled ST sequence, separation
by temperature gradient gel electrophoresis, and densitometric analysis
of autoradiographs (28). For products with 500 CMV DNA
copies in 10 µl the values from the high-ST reaction were used, and
for products with <500 CMV copies those from the low-ST reaction were
used. Results were expressed as the average value of two measurements,
which differed by 15% (data not shown). Exact quantification was
possible within the ranges of 5 to 104 CMV wild-type genome
and 2 × 103 to 2 × 105 -globin
copies per PCR.
In mixed PBL, CMV/cellular DNA ratios were expressed as CMV
copies/2 × 105 copies of -globin (the theoretical
maximum DNA yield from 105 cells). To allow precise
comparison of CMV DNA levels in PMNL and PBMC, CMV DNA copies were
related to the expected -globin DNA copy numbers present in the
mixed PBL population. For example, if 6 × 104 PMNL
were counted in 105 mixed PBL, the theoretical maximum
cellular DNA yield from PMNL was 1.2 × 105 copies of
-globin. Thus, in this case the CMV/-globin ratio in the PMNL
fraction was expressed as CMV copies/1.2 × 105 copies
of -globin.
Plasma CMV copy numbers were expressed as CMV genome equivalents
present in 10 µl of plasma (approximately equivalent to the volume of
whole blood containing 105 PBL).
Statistical analysis.
Frequencies of PCR-positive results
among different leukocyte subsets were compared by McNemar's test.
Frequencies of PCR-positive results for plasma were compared by the
2 test. Correlation of pp65 antigen-positive cells and
CMV DNA levels in leukocyte subsets was determined by Spearman
regression analysis. Differences in pp65 antigen-positive cell counts
and in CMV copy numbers between different groups of patients were tested for significance by the Mann-Whitney U test. In all test procedures P values <0.05 were considered to be
statistically significant.
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Active CMV infections. Twenty-three of the 40 CMV IgG-positive patients developed CMV infections as confirmed by pp65 antigenemia. Eighteen patients, of whom 10 were considered to be symptomatic, were treated with ganciclovir. Four patients (of whom three showed other CMV-associated symptoms) experienced steroid-resistant graft rejection concomitant with pp65 antigenemia and were therefore additionally treated with ATG and OKT3.
A total of 43 pp65 antigen-positive specimens were obtained prior to antiviral treatment. Thirty additional samples were antigen positive after onset of ganciclovir therapy. Sixty samples were obtained from the remaining 17 patients with no evidence of active CMV infection.Qualitative CMV PCR. All 73 antigen-positive samples (before or during therapy) tested positive by qualitative PCR for all leukocyte fractions (Table 1). All patients became pp65 antigen negative within the first week of ganciclovir therapy, which paralleled clinical recovery within 10 days. Of 55 pp65-negative samples analyzed up to 7 weeks after onset of treatment, 47 mixed-PBL samples (85.5%) (Table 1) and 45 PBMC samples (81.8%) were still CMV PCR positive. In contrast, consistent with clinical recovery, only four PMNL specimens (7.3%) remained positive (P < 0.001).
|
CMV DNA levels in patients with active CMV infection. For the 73 pp65 antigen-positive samples CMV DNA copy numbers in the leukocyte subsets and plasma were determined (Table 2). Antigen-positive counts varied between 4 and 563 (median, 152) cells/105 PBL in the 43 samples drawn from patients before onset of ganciclovir treatment and were significantly lower in the 30 samples obtained during therapy (range, 5 to 122; median, 26) (P < 0.001).
|
0.150; P = 0.20)
(Fig. 1A). The same relationship was
observed during antiviral treatment between pp65 antigen-positive cell counts and CMV DNA copies in mixed PBL (rS = 0.964; P < 0.001) and PMNL (rS = 0.958; P < 0.001) but not in PBMC
(rS = 0.068; P = 0.25) (Fig.
1B). The higher the CMV DNA load in PMNL, the more negligible was the
difference in CMV copies in mixed PBL, due to the constant low levels
of CMV genome copies in PBMC.
|
CMV DNA levels in patients with latent CMV infection. In PBMC, no differences in CMV DNA load were detectable between patients with active CMV infection and those with latent CMV infection (Table 2). In contrast, the CMV DNA copy numbers were significantly lower in mixed PBL (P < 0.001) and PMNL (P < 0.001) of latently infected patients than in those of patients with active CMV infection and positive pp65 antigenemia. When pp65 antigenemia was negative after ganciclovir therapy of patients with active CMV infection, no significant differences in CMV DNA copy numbers were found in mixed PBL, PMNL, and PBMC compared to patients with latent infections.
Similarly to CMV DNA levels in mixed PBL and PMNL, in plasma samples from patients with latent infection CMV DNA levels were significantly lower (P < 0.001) than in pp65 antigen-positive samples (Table 2). No significant differences were noted in comparison to pp65 antigen-negative samples after ganciclovir treatment.| |
DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
|
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In our setting PBMC (monocytes and/or lymphocytes) must be regarded as the main source of unwanted positive results by qualitative PCR in pp65 antigen-negative samples. In pp65 antigen-negative patients who had clinically recovered after antiviral therapy as well as in latently infected patients the rate of detection CMV DNA in PMNL was significantly lower than the rate of detection in PBMC, which is compatible with reports that in latently infected patients PBMC harbor CMV DNA in the nuclei more frequently than PMNL (5, 22, 37). Even if PMNL were not infected at all, small-scale contamination of the Ficoll-purified PMNL fractions with monocytes and/or lymphocytes could cause positive PCR results.
CMV DNA copy numbers in PBMC determined by quantitative PCR were equally low in pp65 antigen-negative patients and in actively infected individuals, and no reduction kinetics were seen during antiviral therapy. This suggests that the detected CMV genomes reflected abortive infection. However, deviant observations have been reported (3, 27): some immunocompromised patients with active CMV infection showed high CMV DNA copy numbers in PBMC. Although not statistically significant, ganciclovir induction treatment has been shown to reduce the number of CMV genome copies in PBMC (3). The reasons for these discrepant findings are unclear. One possibility is that patients with primary CMV infections were enrolled in the above studies, whereas in our setting only patients with secondary CMV infections were monitored. During primary virus dissemination PBMC might play a more important role than in secondary infection. On the other hand, differences in cell tropism among viral strains should also be considered.
A high correlation has been described between pp65 antigen-positive cell counts and overall CMV DNA copies in mixed PBL detected by a hybrid capture system (23, 38). However, the quantitative distribution of CMV DNA among leukocyte subpopulations was not considered in these previous investigations. Utilizing quantitative PCR, we observed that solely CMV DNA copy numbers in the PMNL were responsible for the positive correlation with pp65 antigenemia. Firstly, pp65-positive samples showed significantly higher CMV DNA load in mixed PBL and in PMNL than pp65-negative samples. The mean differences in CMV DNA load in mixed PBL and PMNL were negligible due to the constantly low CMV DNA copy numbers in PBMC. Furthermore, the sharp decline of CMV DNA genomes in the mixed PBL fraction during antiviral therapy, which has also been noted by others (3, 9, 10), accompanied by rapid clinical recovery of patients with symptomatic infections, could be attributed to PMNL alone as well. Thus, CMV DNA copies in PMNL of pp65 antigen-negative patients following therapy showed no difference from the levels in PMNL of latently infected patients. Since the same high correlation between CMV DNA levels in mixed PBL or PMNL and pp65 antigen-positive cells could be observed before and during therapy, this would suggest that elimination kinetics are similar for both parameters. Considering the much higher stability of CMV DNA compared to pp65 antigens in blood samples processed with delay (30), CMV DNA quantitation in mixed PBL must be regarded as a promising alternative to the pp65 antigenemia assay.
Our findings add to the evidence that viral DNA detected in PMNL is associated with active CMV infection. This is supported by the fact that in patients who became symptomatic significantly higher peak CMV DNA levels were observed in the PMNL. However, de novo virus production seems to occur mainly at surrounding sites of replication (12, 14, 17, 22) and not, or probably to a much lesser extent (13, 39), in the PMNL themselves. Although only 1 to 4% of pp65 antigen-positive PMNL have been reported to harbor CMV DNA (17), we found CMV DNA by PCR in all PMNL preparations from actively infected patients. The fact that CMV genomes were detected in all PMNL fractions of low-level antigenemic samples may have been due in part to the presence of abortively infected PMNL or to small-scale contamination with infected PBMC. On the other hand, endothelium-derived cells carrying CMV DNA, which have been found in Ficoll-purified PMNL and PBMC fractions (15) during active CMV infection, also might have contributed to the positive PCR results. However, this was not likely to be a major reason for the high correlation of pp65 antigen with CMV DNA we observed in PMNL, since we found no increased percentage of atypical cells in Giemsa stains of PMNL fractions from high-level pp65-antigenemic patients.
In recent years CMV PCR for plasma has been proposed by various investigators (7, 24, 32). Advantages over analysis of leukocytes are seen in the fact that plasma is comparatively easy to process and that higher specificity of positive results with respect to active CMV infection has been reported. However, the exact character of DNA detectable in plasma is still controversial. Although infectious virus has occasionally been recovered from plasma (10, 32), shedding of CMV DNA from lysed leukocytes into the plasma is also a possible explanation (41). Although the CMV DNA remains detectable after ultrafiltration, cellular DNA is also routinely detected in the same samples (10). It is probable that the outcome of plasma PCR strongly varies with the DNA preparation method used. Therefore, more investigations are needed to precisely characterize the CMV DNA detectable in plasma samples.
In our setting positive CMV PCR from plasma was highly associated with active CMV infection. Although less sensitive than mixed-PBL PCR for identifying active infection, quantitative analysis revealed significantly higher peak levels in symptomatic than in asymptomatic patients, similar to leukocyte DNAemia. This has been also described by others for AIDS patients (10, 31), although for unknown reasons Gerna et al. (10) observed only low-level plasma DNAemia in solid-organ transplant recipients with CMV disease.
During antiviral therapy significant decline of plasma DNAemia was detectable. Furthermore, unwanted positive results in pp65-negative samples occurred in plasma with lower frequency than in mixed PBL. However, in comparing PCR for plasma with PCR for the purified leukocyte fractions the situation was different. PCR for PMNL was more sensitive for active infection than PCR for plasma and produced positive results in all samples still positive for pp65 antigens during antiviral treatment, whereas negative plasma PCR results were obtained in 38% of these samples.
Interestingly, in pp65-negative samples (after therapy or in latently CMV-infected patients) the frequency of positive PCR results was lower in PMNL than in plasma, although the difference was not statistically significant. The reasons for this are not clear, but the most likely explanation is that cell debris of latently CMV-infected PBMC contaminated plasma fractions, since the CMV copy numbers detected in plasma of pp65-negative samples were low and we did not subject plasma samples to ultrafiltration. Low copy numbers of cellular DNA in the plasma were also regularly detectable.
In summary, we demonstrated that analysis of leukocytes by qualitative CMV PCR to monitor secondary CMV infection and antiviral therapy in renal-allograft recipients is feasible only if purified PMNL are used. In our setting we observed higher sensitivity of PMNL PCR in pp65-positive samples but fewer unwanted positive PCR results in pp65 antigen-negative samples compared to corresponding plasma preparations.
On the other hand, mixed PBL are sufficient for use in quantitative PCR, since during active infections the differences between mixed PBL and PMNL in CMV DNA load become negligible due to the low copy numbers of nonpredictive CMV DNA in PBMC. Furthermore, due to the higher sensitivity, PBL might be superior to plasma for use in quantitative CMV PCR to monitor CMV therapy and to screen for CMV relapse.
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ACKNOWLEDGMENT |
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We thank Dietrich Mack for critically reviewing the manuscript.
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FOOTNOTES |
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* Corresponding author. Mailing address: Institut für Medizinische Mikrobiologie und Immunologie, Universitäts-Krankenhaus Eppendorf, Martinistr. 52, D-20246 Hamburg, Germany. Phone: (49-40) 4717-3157. Fax: (49-40) 4717-4881. E-mail: pschaefe{at}uke.uni-hamburg.de.
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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|---|
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), PMNL (x) and PBMC (
) of patients with
active CMV infection determined by Spearman regression analysis. (A)
Forty-three samples from 23 patients were analyzed before onset of
ganciclovir therapy. Significant correlation was observed for mixed PBL
(rS = 0.979; P < 0.001) and
PMNL (rS = 0.973; P < 0.001)
but not for PBMC (rS =