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Clinical and Diagnostic Laboratory Immunology, September 1998, p. 703-710, Vol. 5, No. 5
Eijkman-Winkler Institute for Microbiology,
Infectious Diseases and Inflammation, Section Vaccines, Utrecht
University Hospital, 3584 CX Utrecht, The
Netherlands,1 and
Wyeth-Lederle
Vaccines and Pediatrics, Rochester, New York
14586-97282
Received 18 December 1997/Returned for modification 9 April
1998/Accepted 9 June 1998
A phagocytosis assay for Streptococcus pneumoniae based
on flow cytometry (FACS) with human polymorphonuclear cells and human complement was developed for the study of human vaccination antisera. Human prevaccination sera already contain high levels of
C-polysaccharide (C-PS) antibodies, which are not protective in humans
but which might give false positive results in a flow-cytometry-based
assay. Cultures of S. pneumoniae grown to log phase on
three consecutive days, followed by heat inactivation, yielded stable
and highly encapsulated strains for serotypes 6A, 6B, 14, 19F, and 23F.
As a result, only serotype-specific antibodies were able to facilitate phagocytosis of these strains, whereas no phagocytosis was observed with antibodies against C-PS or pneumococcal surface proteins. No, or
weak, phagocytosis was observed with human prevaccination sera, whereas
in general, postvaccination antisera facilitated phagocytosis. A highly
significant correlation was observed between enzyme-linked
immunosorbent assay titers and FACS phagocytosis titers
(r = 0.98, P < 0.001) for serotype
23F pneumococci with human vaccination antisera. For all serotypes,
interassay variation was below 10%. Major advantages of this assay
over the classical killing assay are that (i) limited amounts of sera
are required (10 µl per titration curve), (ii) 600 samples can be
processed in one day by one person, and (iii) cells can be fixed and
measurement of the samples can be performed up to 1 week later.
A number of pneumococcal
saccharide-protein conjugate vaccines are currently under development
and entering phase III trials (10, 35). In addition to other
tests (enzyme-linked immunosorbent assays [ELISA], avidity-affinity
tests), the efficacy of these vaccines is ultimately assessed by
comparing the incidence of pneumococcal disease in the vaccinated
versus nonvaccinated group. The incidence of disease caused by
serotypes included in these multivalent vaccines varies, which makes it
difficult to evaluate the efficacy of each component. Moreover, their
composition must be adapted depending on the geographical area and
probably also over time (13, 15, 25). Therefore, the
introduction of this type of vaccine would be enormously facilitated by
the availability of assays measuring in vitro parameters that correlate
with in vivo protection.
Antibody-complement-dependent phagocytosis is the crucial defense
mechanism against Streptococcus pneumoniae. The ability of
serotype-specific antibodies to provide protection against infections
with S. pneumoniae is beyond doubt, whereas the protective capacity of anti-pneumococcal surface protein antibodies remains to be
established (4). The method most commonly used to measure levels of serotype-specific antibodies in the serum is the ELISA. This
method determines the amount and isotype distribution of the antibodies
present, but provides no direct information about antibody function. In
addition, the correlation between antibody titer and protection depends
on the pneumococcal serotype (14, 20, 34). One of the in
vitro parameters that therefore provides essential information about
the functioning of antibodies is their ability to promote phagocytosis
as determined by phagocytosis assays based on flow cytometry (FACS) or
radioactivity or classical killing assays (1-3, 8, 11, 16, 18,
21, 26, 30, 33, 37).
For human vaccination sera, conflicting data for the relation between
antibody response and phagocytosis exist. Most studies have shown a
weak or nonexistent relationship between these parameters (7, 17,
19, 22, 26), although a good correlation has also been reported
(5, 11). These differences can in part be attributed to the
differences in methodology used for measuring phagocytosis, e.g.,
differences in concentrations of bacteria and sera. More important,
however, is the role of anti-cell-wall-polysaccharide (C-PS)
antibodies. C-PS antibodies can mask the relationship between phagocytic activity and antibody concentration. Viôarsson et al.
demonstrated that the correlation between ELISA titers and phagocytosis
titers improved when the antisera were absorbed with C-PS before the
antibody concentration was measured (37). Depending on the
phagocytosis assay conditions, C-PS antibodies can facilitate phagocytosis (36a). C-PS antibodies, however, are not
protective in humans, and human prevaccination sera usually contain
high concentrations of these antibodies (9, 24, 27, 28, 31, 36,
37). Therefore, C-PS antibody-mediated phagocytosis should be
minimized in phagocytosis assays. In principle, this can be achieved by
minimizing the accessibility of C-PS by selecting highly encapsulated
strains. An alternative strategy is to preabsorb the serum with C-PS.
Phagocytosis can be assessed by the classical killing assays and assays
based on radioactivity or FACS. Previously, we developed a pneumococcal
phagocytosis assay for mouse antisera based on FACS (1, 2).
This assay gave an excellent correlation with antibody titers and
protection as measured in a mouse challenge model (3). In
the present study, this assay was adapted for use with human sera
obtained from persons vaccinated with pneumococcal conjugate vaccines.
To determine the best method for minimizing the influence of anti-C-PS
antibodies, the application of highly encapsulated strains and
preabsorption of antisera with C-PS was evaluated. Highly encapsulated
strains (serotypes 6A, 6B, 14, 19F, and 23F) were obtained by growing
pneumococcal strains to log phase on three consecutive days
(28). As a result, only serotype-specific antibodies were
able to promote phagocytosis of these strains. Using these strains, our
FACS-based phagocytosis assay gave an excellent correlation with ELISA
antibody concentrations. Our assay is now operational for the pediatric
pneumococcal serotypes 6A, 6B, 14, 19F, and 23F, but can easily be set
up for other serotypes when required.
Growing of bacteria.
S. pneumoniae serotypes 6A,
6B, 14, 19F, and 23F (ATCC strains; a kind gift of J. Henrichsen
and U. B. Sørensen, Statens Seruminstitut, Copenhagen, Denmark)
were plated on blood agar plates and grown overnight at 37°C in a 5%
CO2 atmosphere. Three milliliters of Todd-Hewitt broth
supplemented with 0.5% yeast extract (E. Merck Mikrobiologie,
Darmstadt, Germany) was then inoculated with the strains (optical
density at 660 nm [OD660] of 0.05 to 0.08). Bacteria were
grown either to log phase, to stationary phase, or to log phase three
times in order to obtain highly encapsulated strains. For growing
bacteria three times to the log phase, 3 ml of Todd-Hewitt broth
supplemented with 0.5% yeast extract and 5% heat-inactivated human
pooled serum was inoculated with S. pneumoniae
(OD660 of 0.05 to 0.08). Cultures were grown 4 to 5 h
to the log phase (OD660 of approximately 0.5) and then
stored overnight at 4°C. For the second culture, 3 ml of fresh medium
was inoculated with the previous culture (OD660 of
approximately 0.5), grown to the log phase, and stored overnight at
4°C. Likewise, a third culture was started from the second culture
and grown to the log phase. Absence of contamination by other organisms
was checked by plating the bacteria on blood agar plates. Bacteria from
the third culture were washed once with phosphate-buffered saline (PBS)
(2,520 × g, 15 min, 4°C) and resuspended in PBS to
an OD660 of 1.0.
Inactivation of S. pneumoniae strains.
Before
and after inactivation, the bacteria were resuspended in PBS to an
OD660 of 1.0 (approximately 109 bacteria/ml).
Three different methods were evaluated for the inactivation of the
pneumococcal autolysins. The first was formaldehyde killing, in which
formaldehyde (54 µl per ml of bacterial suspension) was added slowly
with stirring. Bacterial suspensions were incubated for 1 h at
37°C, centrifuged, and washed twice with PBS. The second was heat
killing, in which bacterial suspensions were incubated for 1 h at
60°C and washed once with PBS. The third method was killing with 70%
ethanol, in which bacteria were spun down and resuspended in the same
volume with 70% ethanol. After incubation for 1 h at 4°C, the
bacteria were washed twice with PBS.
Fluorescence labeling of pneumococcal strains.
Bacteria were
labeled with a 0.5-mg/ml solution of fluorescein isothiocyanate (FITC,
Isomer I; Sigma Chemical Co., St. Louis, Mo.) in PBS for 1 h at
4°C. Bacteria were washed twice with Hanks' balanced salt solution
containing 1% bovine serum albumin (BSA-HBBS), resuspended in BSA-HBSS
to an OD660 of 1.0, and stored at Rabbit antisera.
Adult female New Zealand White rabbits of
about 3 kg were supplied by Iffa-Credo, Someren, The Netherlands, and
maintained at the Central Laboratory of Experimental Animals (Utrecht
University, Utrecht, The Netherlands). These rabbits were immunized
subcutaneously at four sites with a total of 100 µg of a
C-polysaccharide-keyhole limpet hemocyanin conjugate in Freund's
complete adjuvant (the ratio of polysaccharide to protein was 0.6;
volume, 0.8 ml). A booster injection was given at day 22, and serum was
obtained at day 31 (titer, 105, as determined by ELISA).
Other rabbits were injected with serotype 6B, 14, 19F, or 23F
formalin-killed S. pneumoniae in Freund's complete adjuvant
(total volume, 0.8 ml). Booster injections were given intraperitoneally
in incomplete Freund's adjuvant at days 14, 21, and 28 after the first
immunization with 5 × 108, 1 × 109,
and 5 × 109 bacteria, respectively. After 2 months'
rest, the immunization scheme was repeated. The rabbits were bled at
days 0, 14, 35, 57, and 112 after the first immunization. Rabbit
anti-pneumococcal protein antisera were kindly provided by Karin
Overweg, Laboratory of Pediatrics, Erasmus University, Rotterdam, The
Netherlands. These rabbits were injected and boosted with pneumococcal
serotypes 4 and 19F hydrophobic protein fractions.
Human antisera.
Human pneumococcal S6A and S23F bivalent
conjugate antisera were kindly provided by Wyeth-Lederle Vaccines and
Pediatrics, Rochester, N.Y. Human antisera used for the evaluation of
the reproducibility of the assay were a generous gift of G. Rijkers, Department of Immunology, Wilhelmina kinderziekenhuis, University Hospital for Children and Youth, Utrecht, The Netherlands. All sera
were heated at 56°C for 30 min to inactivate complement components.
Isolation of human complement.
Human pooled serum was
depleted of immunoglobulin G (IgG) by protein G affinity chromatography
(Pharmacia Biotech, Roosendaal, The Netherlands) and stored at
Isolation of human PMN cells.
Human polymorphonuclear (PMN)
cells were isolated from the blood of healthy volunteers. A total of 30 ml of heparinized blood of a single donor was mixed with 30 ml of PBS
(pH 7.4), layered on Ficoll-Histopaque gradient, and centrifuged for 20 min at 400 × g. The cell pellet, containing PMN cells
and erythrocytes, was depleted of erythrocytes by two consecutive
hypotonic shocks (6).
Phagocytosis assay.
The assay was adapted from Alonso de
Velasco et al. (1, 2). In short, dilutions of
heat-inactivated serum and complement, which was diluted to a fixed
concentration of 2% (final concentration in the assay), were made in
BSA-HBSS and pipetted into round-bottomed microtiter plates (Greiner
Labortechnik, Alphen aan de Rijn, The Netherlands). Samples of 2.5 × 106 pneumococci were added to each well. Opsonization
was performed in a total volume of 50 µl at 37°C with shaking on a
microtiter plate agitator. After 30 min of opsonization, the plates
were placed on ice and 2.5 × 105 PMN cells in 50 µl
of BSA-HBSS were added to each well. Phagocytosis was performed for 30 min at 37°C with shaking. An incubation time of 30 min leads to
ingestion of all adherent pneumococci (29). After a wash
with ice-cold BSA-HBSS, the cells were transferred to FACS tubes, fixed
with paraformaldehyde (2%) in PBS, and analyzed in a flow cytometer
(FACScan; Becton Dickinson, Mountain View, Calif.). The percentage of
FITC-positive PMN cells was used as a measure of the phagocytic
activity of serum. Percentages of FITC-positive PMN cells were
corrected for the percentage of FITC-positive PMN cells of the negative
control (without antiserum) (Fig. 1). Results are expressed as 25% phagocytosis titers, calculated by linear
regression as the serum dilutions resulting in 25% FITC-positive PMN
cells.
1071-412X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Use of Highly Encapsulated Streptococcus
pneumoniae Strains in a Flow-Cytometric Assay for Assessment of
the Phagocytic Capacity of Serotype-Specific Antibodies
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
20°C in 100-µl
amounts (108 bacteria).
70°C. Depleted sera did not contain detectable IgG levels
(LC-Partigen IgG, Behringwerke AG, Malburg, Germany), and complement
activity (as determined by a CH50 assay [23]) was
conserved for at least 60% of each portion compared to undepleted
source serum.
View larger version (18K):
[in a new window]
FIG. 1.
(a) PMN cell gating (R1) based on their specific forward
(FSC) and right angle (SSC) light scatter. (b) Analysis of phagocytosis
of fluorescence-labeled S. pneumoniae by PMN cells. The
histograms show FITC-positive and -negative PMN cells (discriminated by
marker M1) for different serum concentrations: 10% (A), 2% (B), 0.4%
(C). Negative controls: PMN cells without serum (D), PMN cells without
serum and complement (E), PMN cells only (F).
phagocytosis titer with inhibitor) × 100%/phagocytosis titer without inhibitor.
ELISA. The ELISA was performed as previously described (32). Serotype-specific polysaccharide was obtained from the American Type Culture Collection (Rockville, Md.) for use as antigen. Specimens were preadsorbed with C-polysaccharide-enriched absorbent prepared by Wyeth-Lederle Vaccines and Pediatrics and quantitated against lot 89SF (Center for Biological Research and Evaluation, Food and Drug Administration, Washington, D.C.).
Statistical analysis. The coefficient of variation was obtained after log transformation by the following formula: (standard deviation/mean) × 100. Correlations between ELISA titers and FACS phagocytosis titers were analyzed by linear regression tests. Statistical significance of correlations was assessed by Student's t test. A P value of <0.05 was considered statistically significant.
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Effect of pneumococcal growth phase on phagocytosis. Most human antisera contain antibodies directed against C-PS of S. pneumoniae (31), which probably facilitate phagocytosis of poorly encapsulated strains. Therefore, in order to develop a serotype-specific phagocytosis assay, highly encapsulated strains are required. First, the effect of the growth phase on encapsulation was examined. To measure the effect of encapsulation, a strain grown to log phase and a strain grown to stationary phase were opsonized with either a rabbit anti-C-PS antiserum or a serotype-specific antiserum, and phagocytosis was measured. The strain grown to log phase displayed relatively low phagocytosis with the C-PS antiserum compared to the capsular polysaccharide antiserum, whereas the strain grown to stationary phase gave strong phagocytosis with the C-PS antiserum compared to the serotype-specific antiserum. Both antisera strongly promoted phagocytosis of the stationary strain, indicating that although the strain is less well encapsulated, its phagocytosis with the serotype-specific antiserum is maintained (Fig. 2A and B).
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) and serotype-specific antiserum (
). (B)
Phagocytosis of log-phase strain with an antiserum against C-PS (
) or
preincubated with C-PS (
). (D) Influence of C-PS preincubation and
the use of the log-phase strain on C-PS antibody-mediated phagocytosis.
C-polysaccharide antiserum was used alone (C-PS preincubation. In order to diminish the influence of C-PS antibodies on phagocytosis, anti-C-PS antisera were preincubated with C-PS. Phagocytosis assays were subsequently performed with a stationary-phase strain (Fig. 2C) and a log-phase strain (Fig. 2D). For strains grown to both phases, C-PS antibody-mediated phagocytosis was strongly reduced by this preincubation. In contrast, no effect was observed for the phagocytosis mediated by the serotype-specific antiserum (data not shown). However, in general, complete preabsorption of C-PS antibodies with C-PS was difficult to achieve. Therefore, another method was investigated for eliminating the influence of C-polysaccharide antibodies in the FACS-based assay.
Strains grown to log phase three times. Nielsen et al. described a method for obtaining highly encapsulated strains by growing strains to log phase three times consecutively (28). Such highly encapsulated strains were tested in the phagocytosis assay with both the serotype-specific and anti-C-PS antisera. The serotype-specific antiserum strongly promoted phagocytosis, whereas almost no phagocytosis was observed with the anti-C-PS antiserum (Fig. 3). Identical results were obtained for serotypes 6A, 6B, 14, and 23F (data not shown).
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Inactivation.
When live strains were used, some C-PS
antibody-mediated phagocytosis was observed in some of the experiments.
S. pneumoniae produces enzymes (autolysins) that can cause
lysis of the bacterium and probably also partial release of the capsule
(12). Killing the bacteria leads to inactivation of these
enzymes (12). Three different methods for killing the
pneumococci were evaluated: heat inactivation, killing by ethanol, and
killing by formaldehyde. Heat inactivation and formaldehyde treatment
both resulted in the absence of phagocytosis with anti-C-PS antibodies,
whereas with ethanol treatment some residual phagocytosis was detected (Fig. 4). The strongest phagocytosis with
the serotype-specific serum, however, was observed when heat
inactivation was used. Therefore, subsequent experiments were performed
with heat-inactivated strains grown to log phase three times. Strains
treated in this way can be stored at 20°C for at least half a year
without losing the properties described above (data not shown).
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Anti-protein antibodies. In addition to C-PS antibodies, human antisera are expected to contain antibodies to surface proteins of S. pneumoniae. Encapsulation will probably influence the ability of these anti-protein antibodies to facilitate phagocytosis. To investigate this possibility, rabbit pre- and postvaccination sera against hydrophobic pneumococcal proteins of serotypes 4 and 19F pneumococci were used. A serotype 19F strain was grown either to stationary phase or to log phase three times and heat inactivated. The anti-protein antiserum was only able to promote phagocytosis of the stationary grown strain, whereas no phagocytosis was observed with the strain grown to log phase three times (Fig. 5).
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Capsular polysaccharide preincubation. To demonstrate that only serotype-specific phagocytic antibodies are detected when heat-inactivated strains grown to log phase three times are used, sera were absorbed with serotype-specific polysaccharide or C-PS. For all serotypes, preincubation of the serotype-specific serum with serotype-specific polysaccharides resulted in a strong inhibition of phagocytosis, whereas no inhibition was observed after serum absorption with C-PS (Fig. 6).
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Correlation with ELISA. Phagocytosis of pneumococci is mediated by antibodies in cooperation with complement. To investigate the relationship between antibody concentration and phagocytosis titer, antibody concentrations and phagocytosis titers were determined in 46 human pre- and postvaccination antisera. Sera were heat inactivated, and human IgG-depleted pooled serum was used as an exogenic complement source (Fig. 7). No, or weak, phagocytosis was observed for prevaccination sera, whereas, in general, postvaccination antisera gave phagocytosis. A strong, highly significant correlation was observed between IgG antibody concentrations and phagocytosis titers (r = 0.98, P < 0.001). Without complement, similar results were obtained (r = 0.97), but no phagocytosis was observed for prevaccination antisera (data not shown).
|
) and postvaccination
(
) sera. ELISA titers and phagocytosis titers were determined for 48 pre- and postvaccination antisera.
Coefficient of variation. The reproducibility of the phagocytosis assay for each serotype was determined by measuring the phagocytosis titers of a serotype-specific rabbit antiserum and a human conjugate vaccine antiserum on five different days. For all serotypes, with rabbit antisera, interassay variation was below 5%, whereas human antisera gave an interassay variation below 10% (Table 1).
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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This report describes a pneumococcal phagocytosis assay which predominantly measures phagocytosis mediated by serotype-specific antibodies. Rabbit hyperimmune antisera directed against either C-PS or surface proteins failed to promote phagocytosis in this assay. Moreover, in contrast to C-PS, only preincubation of the sera with serotype-specific polysaccharide could inhibit phagocytosis.
The accessibility of C-PS on pneumococci was minimized by selecting for highly encapsulated strains. This was achieved by growing the strains three times to the log phase in the presence of 5% human pooled serum (HPS). A possible mechanism for the effect of this procedure is that C-PS antibodies present in the HPS cause agglutination and thereby inhibit growth of poorly encapsulated strains. In this way, each subsequent culture is enriched with highly encapsulated pneumococci. To ensure that every experiment was performed with highly encapsulated pneumococci, stocks of pneumococci were regularly tested for the absence of phagocytosis with the rabbit anti-C-PS antiserum. Therefore, anti-C-polysaccharide antiserum can be used as an easy quality control for strain encapsulation.
When live, highly encapsulated bacterial stocks were used, particularly those of strain 23F, appearance of C-polysaccharide antibody-mediated phagocytosis was observed after freezing and thawing, probably due to the release and activation of pneumococcal enzymes (autolysins). Comparing methods for inactivating these enzymes, such as heat treatment, ethanol fixation, and paraformaldehyde fixation, indicated that heat inactivation for 1 h at 60°C gave the best results (Fig. 4). Strains treated this way gave no phagocytosis with the anti-C-polysaccharide antiserum and the strongest phagocytosis with the serotype-specific antiserum. A potential disadvantage of the use of heat treatment is the potential denaturation of protein epitopes on the pneumococcus. Therefore, when the purpose is to evaluate the opsonic capacity of anti-pneumococcal protein antibodies, live and heat-inactivated strains should initially be compared.
Interassay variation of the FACS-based assay was excellent and in the
same range as that recently reported for the classical killing assay in
which HL-60 cells were used as a source of phagocytes (33).
With rabbit antisera, the interassay variation was below 5% for all
serotypes, whereas with human antisera, an interassay variation of
around 10% was observed (Table 1). Part of this difference is probably
due to Fc
polymorphisms on the PMN cells used. For testing of the
human antisera, care was taken to use donors who were either
heterozygous or homozygous for FcRIIa-131H. These donors, however,
possessed different FcRIIIb receptors, which affects the
phagocytosis mediated by IgG1 and IgG3 antibodies (NA1/NA2). Rabbits
produce only a single type of IgG, and as far as we know, the
interaction with human FcRIIa and FcRIIIb is not dependent on the
polymorphisms of these receptors. The influence of FcRIIa and
FcRIIIb polymorphisms on the performance of the phagocytosis assay
is currently under investigation in our laboratory.
To evaluate the performance of the FACS-based assay with human antisera, the phagocytic capacities of pre- and postvaccination sera obtained from adults vaccinated with various conjugate vaccines or Pneumovax were determined. Independent of antibody concentrations, no phagocytosis was observed for prevaccination antisera without addition of complement, suggesting that these prevaccination sera probably contained phagocytic IgM antibodies. Comparison of the FACS-based phagocytosis titers and the IgG antibody concentrations demonstrated a strong and highly significant correlation between these two parameters. In this respect, the FACS-based phagocytosis assay adapted for use of human antisera displayed characteristics identical to those of our previously described assay for mouse antisera, in which we used the J774 mouse cell line (2, 3). This assay not only correlated strongly with the serotype-specific IgG and IgM antibody levels but was (in combination with the IgG antibody levels) also the best predictor of survival of vaccinated mice upon challenge with a lethal dose of pneumococci (3).
The classical killing assay is considered to be the "gold standard" for the assessment of the phagocytic capacity of antisera. That assay, however, is cumbersome to perform, only a limited number of antisera (at most 30) can be processed per assay, and the test has to be evaluated the next day (33). With the FACS-based assay, 600 samples (150 antisera/4 serum dilutions) can be processed in 1 day by one person. Moreover, the cells can be fixed and the flow cytometry can be performed up to 1 week later. In addition, in the FACS-based assay, the results are measured by a machine and analyzed by computer, whereas with the classical killing assay, the colonies are scored by eye, leading more easily to human errors. Moreover, the use of antibiotics by patients or vaccinated people affects the outcome of the killing assay. The FACS-based assay uses inactivated strains and is therefore not affected by the presence of antibiotics.
Upon comparison of our FACS-based assay with the killing assays described in the literature, at first sight, our FACS-based assay seems to be less sensitive (33). There are, however, essential differences between both assays. To avoid bacterial outgrowth, effector/target ratios used in classical killing assays vary from 100:1 to 500:1, and baby rabbit serum is utilized as the complement source. The FACS-based assay uses an effector/target ratio of 1:10 and human complement. At the moment, it is difficult to establish what type of assay correlates best with in vivo protection in humans or animals, but effector/target cell ratios during pneumococcal infections of 100:1 to 500:1 seem to be less likely compared to an effector/target ratio of 1:10. In addition, the FACS-based assay for mouse antisera is an excellent predictor of the survival of vaccinated mice after challenge with pneumococci (3). The question raised above, however, can probably be answered only at the end of the current phase III pneumococcal conjugate trials. Large numbers of antisera have to be evaluated for their phagocytic capacity by both assays, and the correlation with protection has to be established. In particular, sera obtained from toddlers who are infected with S. pneumoniae despite having being vaccinated will be important to study. At the moment, we are in the process of setting up interlaboratory studies on the correlation between FACS phagocytosis titers and classical killing titers.
In conclusion, the FACS-based assay is an easy-to-perform method for measuring the phagocytic capacity of large numbers of pneumococcal vaccine antisera. It has low interassay variation and displays a good correlation with postvaccination IgG concentrations.
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ACKNOWLEDGMENTS |
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We thank G. Rijkers, Department of Immunology, Wilhelmina
kinderziekenhuis, University Hospital for Children and Youth,
Utrecht, and K. Overweg, Laboratory of Pediatrics, Erasmus
University, Rotterdam, for providing antisera; J. van der Winkel and N. Westerdaal, Department of Immunology, Utrecht University Hospital,
Utrecht, The Netherlands, for providing the facilities and help for
typing the donors for their FcRIIa and FcRIIIb allotypes; J. Henrichsen and U. B. Sørensen, Statens Seruminstitut, Copenhagen,
Denmark, for their advice on how to obtain highly encapsulated
pneumococcal strains; and C. Kraaijeveld for helpful advice and careful
reading of the manuscript.
This research was funded in part by the World Health Organization, Global Program for Vaccines and Immunization, Vaccine Research & Development (V23/181/92).
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FOOTNOTES |
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* Corresponding author. Mailing address: Eijkman-Winkler Institute for Microbiology, Infectious Diseases and Inflammation, Section Vaccines, Utrecht University Hospital, Rm. G04.614, Heidelberglaan 100, 3584 CX Utrecht, The Netherlands. Phone: 31-30-2506533. Fax: 31-30-2541770. E-mail: W.T.M.Jansen{at}lab.azu.nl.
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Abstract
Introduction
Materials & Methods
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Discussion
References
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Clinical and Diagnostic Laboratory Immunology, September 1998, p. 703-710, Vol. 5, No. 5
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