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Previous Article | Next Article 
Infect Immun, February 1998, p. 794-799, Vol. 66, No. 2
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Growth of Virulent and Avirulent
Mycobacterium tuberculosis Strains in Human
Macrophages
Ming
Zhang,1
Jianhua
Gong,1
Yuanguang
Lin,2 and
Peter F.
Barnes1,3,4,*
Center for Pulmonary and Infectious Disease
Control,1
Department of
Medicine,3 and
Department of Cell
Biology,4
The University of Texas Health
Center at Tyler, Tyler, Texas 75710, and the Department of
Medicine, University of Southern California School of Medicine, Los
Angeles, California 900332
Received 22 July 1997/Returned for modification 24 October
1997/Accepted 20 November 1997
 |
ABSTRACT |
Mycobacterium tuberculosis H37Rv causes progressive
disease in animals, whereas the H37Ra strain does not. The relevance of this difference in virulence to human infection is uncertain because these strains have been shown to have similar growth rates in human
macrophages. To evaluate the intracellular growth of M. tuberculosis strains in macrophages under conditions similar to those encountered in vivo, we infected human monocyte-derived macrophages with H37Ra, H37Rv, or one of four isolates from
tuberculosis patients at a low bacillus-to-macrophage ratio. H37Rv and
the patient isolates grew significantly faster than H37Ra, based on the
numbers of CFU and acid-fast bacilli. These findings did not result
from extracellular mycobacterial growth, differential macrophage viability, or bacillary clumping. In contrast to other published results, these findings indicate that the virulence characteristics of
M. tuberculosis strains in animal models are relevant
to human tuberculosis infection.
| |
INTRODUCTION |
A central issue in the pathogenesis
of tuberculosis is the characterization of virulence determinants of
Mycobacterium tuberculosis that are relevant to human
disease. In guinea pigs and mice, the M. tuberculosis
H37Rv strain is substantially more virulent than the attenuated H37Ra
strain (1, 7). Because the manifestations of tuberculosis in
guinea pigs and mice differ significantly from those in humans, it is
uncertain if the difference in virulence between these two strains is
relevant to human infection with M. tuberculosis.
Furthermore, a recent study found that H37Ra and H37Rv grew at similar
rates in human monocyte-derived macrophages, whereas H37Rv grew more
rapidly in murine macrophages (8).
Quantitation of the intracellular growth of M. tuberculosis in human macrophages is technically demanding for
several reasons. First, M. tuberculosis can destroy
macrophages during the culture period, artifactually reducing the
number of CFU in macrophage lysates. Second, the extracellular growth
of M. tuberculosis may complicate the interpretation of
results. Third, the clumping of M. tuberculosis is most
marked for virulent strains and can artifactually reduce the number of
CFU. To determine the growth characteristics of virulent and attenuated
M. tuberculosis strains in human macrophages under
conditions that mimic those in vivo, we infected monocyte-derived
macrophages with very low concentrations of M. tuberculosis. This strategy minimized the effects of M. tuberculosis on macrophage viability and ensured that an adequate population of macrophages would allow continued intracellular mycobacterial growth.
| |
MATERIALS AND METHODS |
Preparation of monocyte-derived macrophages.
Peripheral
blood mononuclear cells were isolated from buffy coat preparations by
differential centrifugation, first over Ficoll-Paque (Pharmacia Fine
Chemicals, Piscataway, N.J.) and then on Percoll gradients (Pharmacia,
Uppsala, Sweden), and the monocyte fraction was plated in 24-well
plates (Becton Dickinson, Lincoln Park, N.J.) at 5 × 105 cells/well in RPMI medium (GIBCO, Grand Island, N.Y.)
containing 10% heat-inactivated human serum. After 2 h, cells
were washed three times with RPMI medium to remove nonadherent cells.
Adherent cells were 90 to 95% monocytes, based on Giemsa and
nonspecific esterase stains. Adherent cells were cultured in 1 ml of
RPMI medium with 10% heat-inactivated human serum without antibiotics and were allowed to mature into macrophages prior to infection with
M. tuberculosis. At this point, each well contained
approximately 4 × 105 cells, with >95% cell
viability, based on Trypan blue exclusion.
In experiments for which acid-fast staining was performed, monocytes
were cultured on slides in removable chambers (SonicSeal Slide wells;
Nunc Inc., Naperville, Ill.) for 6 days prior to infection with
M. tuberculosis.
Measurement of intracellular mycobacterial growth.
The
M. tuberculosis strains used were two H37Ra isolates
(no. 25177 from the American Type Culture Collection, Rockville, Md., and a second isolate kindly provided by John Belisle, Colorado State University, Fort Collins), one H37Rv isolate (provided by John
Belisle), and four clinical isolates from tuberculosis patients (AS,
ET, S29, and S51). Single-cell suspensions of mycobacteria were
obtained by a modification of standard methods. Briefly, aliquots of
frozen bacilli were cultured in 7H9 media for 7 days, pelleted at
4,500 × g for 15 min, and resuspended in RPMI medium. Clumps of bacilli were dispersed with an ultrasonic cell disrupter (Virtis Co., Gardiner, N.Y.). The sample was centrifuged at 400 × g, and the upper bacterial suspension was used in all
experiments. Bacteria were counted in a Petroff-Hausser chamber. With
this technique, 90 to 95% of the organisms were single bacilli, with the remaining 5 to 10% in small aggregates of up to five organisms. Mycobacterial viability, based on the number of CFU, was 50 to 60% for
all M. tuberculosis strains.
Macrophages were infected in triplicate with M. tuberculosis at 104 bacilli/well. Based on 50%
bacterial viability and an estimated 4 × 105
cells/well, the estimated multiplicity of infection was one live M. tuberculosis organism per 80 cells. After 24 h,
monolayers were washed to remove extracellular bacilli, and this time
point was considered day 0. Cells were cultured at 37°C and 5%
CO2 for six additional days. Fresh RPMI medium and 10%
human serum were added at day 6, and the cells were cultured for four
more days. No antibiotics were ever added to the cultures.
We evaluated the growth of M. tuberculosis in
macrophages on day 10 because this provided sufficient time for bacilli
to grow by 2 log units and because macrophage viability was not reduced during this period. The numbers of CFU were determined on day 10 in all
experiments. In some cases, the numbers of CFU were also measured on
day 3 and day 6. The supernatant was aspirated, and macrophages were
lysed with distilled water for 10 min, incubated with 0.07% sodium
dodecyl sulfate (Sigma Chemical Co., St. Louis, Mo.) for 10 min, and
neutralized with 20% bovine serum albumin (Sigma). Bacterial
suspensions in cell lysates and supernatants were ultrasonically
dispersed, serially diluted, and plated in triplicate on 7H10 agar
plates, and CFU were counted after 3 weeks. The numbers of CFU reported
for days 0, 3, and 6 represent CFU obtained from cell lysates. For days
3 and 6, the numbers of CFU in supernatants were 10- to 20-fold lower
than those in cell lysates. CFU numbers reported for day 10 include CFU
from both the supernatant and cell lysate, because at this time point a
significant proportion of the macrophages were nonadherent and were
present in the supernatant. These macrophages were viable, as assessed
by Trypan blue exclusion, and when the supernatant was centrifuged at
200 × g to pellet the cells but not the extracellular
bacilli, it was found that >90% of the CFU arose from the cell
pellet. This indicates that essentially all mycobacteria were growing
intracellularly in our experimental system.
In some experiments, macrophage viability after the culture period was
assessed by using 0.25% trypsin (GIBCO BRL, Gaithersburg, Md.) and 1 mM EDTA (GIBCO BRL) for 30 min at 37°C to detach the macrophages,
followed by Trypan blue exclusion to estimate the number and percentage
of viable cells. Acid-fast staining was performed with the fluorescent
auramine-rhodamine stain, according to the manufacturer's instructions
(Medical Chemical Corporation, Santa Monica, Calif.), and mycobacteria
were counted with a fluorescence microscope.
Cytokine production.
In some experiments, supernatants of
macrophages infected with M. tuberculosis were
harvested, aliquoted, and frozen at 
70°C. Concentrations of tumor
necrosis factor alpha (TNF-
), interleukin 10 (IL-10), and IL-12 were
measured by enzyme-linked immunosorbent assay, with antibodies from
Pharmingen, San Diego, Calif. (for TNF- and IL-10) and from Maurice
Gately, Hoffmann-La Roche, Nutley, N.J. (for IL-12). The assay
sensitivity was 20 pg/ml for TNF- and IL-10 and 10 pg/ml for IL-12.
Statistical analysis.
The nonparametric Mann-Whitney rank
sum test was used to compare different groups because the data were not
normally distributed.
| |
RESULTS |
Infection of macrophages with M. tuberculosis.
To
estimate the intracellular inoculum of M. tuberculosis,
macrophages were lysed after 24 h of incubation with H37Ra
(obtained from John Belisle), H37Rv, and two clinical isolates (day 0). The washes used to remove extracellular bacilli were pelleted and
resuspended. Measurement of the numbers of CFU in washes and cell
lysates revealed that approximately 80% of the bacteria were in the
washes and 20% were intracellular. Acid-fast staining revealed that
0.1 to 0.2% of the macrophages contained bacilli. Sixty to eighty
percent of the macrophages each contained one bacillus, and the
remainder each contained two bacilli.
Mycobacterial growth in monocyte-derived macrophages, as measured
by CFU.
Figure 1 shows the growth
curves for H37Ra, H37Rv, and clinical isolate ET in macrophages over 10 days, based on nine experiments. The numbers of CFU in macrophage
lysates were comparable at day 0 for all M. tuberculosis strains (Fig. 1). After 10 days, the mean number of
CFU (± the standard error) of H37Ra was 2.1 × 104 ± 0.4 × 104, compared to 1.7 × 105 ± 0.4 × 105 for H37Rv (P = 0.0001). The
mean number of CFU for clinical isolate ET was 7.7 × 105 ± 1.8 × 105, which was significantly
higher than mean number of CFU for H37Ra (P < 0.0001)
or H37Rv (P = 0.0001). The mean numbers of CFU for the
strains at days 3 and 6 paralleled the findings for day 10. To
determine if the slower intracellular growth of strain H37Ra was an
anomaly of that specific isolate, we evaluated a second H37Ra isolate
(strain 25177 from the American Type Culture Collection) and obtained
identical results (data not shown). As an alternative measure of
mycobacterial growth rates, we calculated the generation times for
these isolates, based on the mean numbers of CFU at day 0 and day 10. The mean generation time for H37Ra was 43.9 h, that for H37Rv was
28.6 h, and that for clinical isolate ET was 24.6 h.
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FIG. 1.
Growth of M. tuberculosis in
monocyte-derived macrophages. Monocyte-derived macrophages were
cultured with H37Ra, H37Rv, and clinical isolate ET for 10 days, and
numbers of CFU were measured at different time points. The values shown
are the means and standard errors for nine separate experiments for
days 0 and 10 and for four experiments for days 3 and 6.
|
|
In seven experiments, the mean number of CFU after 10 days of culture
of a second clinical isolate, AS, was 4.0 × 105 ± 0.6 × 105, which was intermediate between values for
H37Rv and strain ET. In three experiments, the mean numbers of CFU for
two additional clinical strains, S29 and S51, were similar to those for
strain AS and intermediate between those for H37Rv and strain ET (data not shown).
Mycobacterial growth in monocyte-derived macrophages, as measured
by acid-fast staining.
As an alternative measure of mycobacterial
growth, we performed acid-fast staining on macrophages after infection
with four M. tuberculosis strains for 10 days.
Approximately 10,000 macrophages were counted in each of two
experiments, and the numbers of macrophages infected with different
numbers of mycobacteria were counted. The numbers of cells infected
with single bacilli were three- to fivefold higher after infection with
the virulent strains than after infection with H37Ra, and similar
findings were noted for macrophages infected with 2 to 31 bacilli per
cell. Macrophages containing 32 or more bacilli per cell were found
only after infection by H37Rv or the clinical isolates (Fig.
2). The highest numbers of macrophages
infected with 16 or more bacilli were found after infection with
clinical isolate ET, paralleling results obtained by measurement of
CFU.
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FIG. 2.
Frequency distribution of the numbers of bacilli in
macrophages infected with M. tuberculosis.
Monocyte-derived macrophages were cultured with H37Ra, H37Rv, and
clinical isolates AS and ET for 10 days. Acid-fast staining was
performed, and approximately 10,000 macrophages were counted in each
experiment. Panels A and B each represent a separate experiment and
show the numbers of macrophages containing the indicated numbers of
bacilli per cell after 10 days.
|
|
Figure 3 shows
representative photomicrographs of macrophages infected with H37Ra and
H37Rv. At low power, it was seen that H37Rv infected far more
macrophages than H37Ra (Fig. 3A and B). The bacilli were associated
with the cells and were not in the intercellular spaces.
Higher-magnification views confirmed that the large clumps of H37Rv
were intracellular (Fig. 3C).
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FIG. 3.
Photomicrographs of M. tuberculosis
H37Ra (A) and H37Rv (B and C) after 10 days of culture in
monocyte-derived macrophages. Panels A and B are
low-power-magnification views (×100) of M. tuberculosis cells in macrophages after staining with
auramine-rhodamine. The photomicrographs were taken with a fluorescence
microscope equipped with a 470- to 490-nm filter (U-MNB; Olympus,
Tokyo, Japan). Bacilli are bright yellow, and macrophages are dull red.
Panel C shows a high-power-magnification view (×1,000) of
M. tuberculosis H37Rv in macrophages after staining
with auramine-rhodamine. A 510- to 550-nm filter (U-MWG; Olympus) was
used to view the slide. The bacilli are bright yellow, and the
macrophages are green. A different filter was used for panel C because
it permitted a more distinct view of cell and bacillary outlines at
high magnification.
|
|
Evaluation of factors that could cause apparent differences in
intracellular mycobacterial growth.
We considered the possibility
that the differences in growth between H37Ra and virulent M. tuberculosis strains resulted from extracellular growth in culture
medium. In three experiments, mean numbers of CFU declined over 10 days
for H37Ra, H37Rv, and clinical isolates ET and AS grown in RPMI medium
and 10% serum (Fig. 4). Standard errors
were 12 to 40% of mean values and are not shown for clarity. To
determine if macrophage-conditioned medium supported mycobacterial
growth, we cultured the four M. tuberculosis strains in
Transwell inserts in 2-ml wells containing macrophages. The inserts
contained 0.4-µm pores that allow solute diffusion but no contact
between bacilli and macrophages. The numbers of CFU of all
mycobacterial strains declined during 10 days of culture, similar to
results shown in Fig. 4 (data not shown).
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FIG. 4.
Extracellular growth of M. tuberculosis
in culture medium. H37Ra, H37Rv, and clinical isolates ET and AS were
cultured in RPMI medium and 10% serum for 10 days. Mean numbers of CFU
are shown for three experiments. Standard errors ranged from 12 to 40%
of mean values and are not shown for the sake of clarity.
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|
Because our experimental system did not support the extracellular
growth of M. tuberculosis, reduced macrophage viability could decrease the number of cells available and artifactually lower
the number of CFU isolated. Four experiments were performed to assess
macrophage viability after 10 days of culture with medium alone and
after infection with H37Ra, H37Rv, or clinical isolate AS. The mean
numbers of macrophages recovered and their viabilities were similar for
cells cultured in media alone or with the three M. tuberculosis strains (Fig. 5).
Therefore, the reduced growth of H37Ra did not result from excessive
destruction of infected macrophages.
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FIG. 5.
Recovery and viability of macrophages after culture with
M. tuberculosis. Monocyte-derived macrophages (4 × 105 per well) were cultured for 10 days in the presence
of media alone or with H37Ra, H37Rv, or clinical isolate AS. The
numbers of macrophages recovered and their percent viabilities, as
assessed by Trypan blue exclusion, were determined. The values shown
are the means and standard errors for four experiments.
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|
Clumping of mycobacteria can artifactually reduce the number of CFU, so
we evaluated the degree of clumping of H37Ra, H37Rv, and clinical
isolates ET and AS. After growth of these strains in macrophages,
aliquots of bacterial suspensions were stained with auramine-rhodamine
prior to plating. For all strains, 95 to 99% of the bacilli were
single, with the remainder in groups of two or three bacilli. Thus, the
reduced growth of H37Ra was not due to excessive clumping of this
strain.
To determine if there was an intrinsic difference in the growth
characteristics of H37Ra, we cultured H37Ra, H37Rv, and clinical isolates ET and AS in 7H9 media. In four experiments, mean numbers of
CFU for all strains were similar at 6 and 10 days (Fig.
6). Standard errors were 12 to 32% of
mean values and are not shown for clarity.
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FIG. 6.
Growth of M. tuberculosis in 7H9 media.
H37Ra, H37Rv, and clinical isolates ET and AS were cultured in 7H9
media for 10 days. Mean numbers of CFU are shown for four experiments.
Standard errors ranged from 12 to 32% of mean values and are not shown
for the sake of clarity.
|
|
Cytokine production.
To determine if the intracellular growth
rates of virulent and avirulent M. tuberculosis were
related to patterns of cytokine production, we measured concentrations
of TNF-, IL-10, and IL-12 in supernatants of macrophages infected
with H37Ra, H37Rv, and clinical isolate ET. At a ratio of one live
M. tuberculosis organism to 80 cells, no detectable
cytokine concentration was measured in cell culture supernatants after
1 to 10 days of culture, and reverse transcription-PCR showed cytokine
mRNA at background levels (data not shown). To obtain measurable
cytokine concentrations, we repeated the experiments with a ratio of
five live M. tuberculosis organisms per cell. Maximal
cytokine concentrations were present at 24 h. In three
experiments, mean concentrations of TNF- (± standard errors) were
3,607 ± 407 pg/ml for H37Ra, 3,283 ± 523 pg/ml for H37Rv,
and 3,408 ± 707 pg/ml for clinical isolate ET (P > 0.10 for all comparisons). IL-10 and IL-12 concentrations were also
similar in supernatants of macrophages infected with the three strains
(data not shown).
| |
DISCUSSION |
Comprehensive knowledge of the genetic and molecular bases of
virulence is central to understanding the pathogenesis of diseases due
to intracellular pathogens. The virulent M. tuberculosis strain H37Rv and its avirulent counterpart H37Ra have
been studied extensively in animal models, and the genetic and
phenotypic differences between these strains are under intensive
investigation. Nevertheless, no published data indicate that the
differences in virulence between these strains that are observed in
animals are applicable to humans. The current data demonstrate that
H37Rv and M. tuberculosis isolates from patients grow
more rapidly in human macrophages than avirulent H37Ra. This conclusion
was arrived at by measuring numbers of CFU and by counting acid-fast
bacilli in macrophages. Rigorous controls confirmed that these findings
did not result from differential extracellular mycobacterial growth,
macrophage viability, or clumping or from the intrinsic growth
characteristics of the strains. These findings provide strong evidence
that the virulence characteristics of M. tuberculosis
strains in animal models are relevant to human tuberculosis.
In guinea pigs and mice, H37Ra and H37Rv both establish infection in
the lung. Host defenses limit the growth of H37Ra and eventually clear
the infection. In contrast, H37Rv replicates very rapidly and the
infection is not contained (1, 7). H37Rv also grows more
rapidly than H37Ra in murine peritoneal macrophages (8), a
murine macrophage cell line (6), human HeLa cells
(10), and human alveolar cell line A549 (2).
Nevertheless, it is uncertain if the increased virulence of the H37Rv
strain in animal models and in human cell lines is relevant to human tuberculosis because the growth of H37Rv and H37Ra has rarely been
evaluated in human macrophages.
The limited published information on the growth characteristics of
M. tuberculosis strains in human macrophages reflects
the difficulties in establishing a reproducible assay system that eliminates confounding factors. Paul and colleagues observed similar growth rates for H37Ra and H37Rv in human macrophages (8). They used a 1:1 ratio of M. tuberculosis to
macrophages, and numbers of CFU for both M. tuberculosis strains increased by approximately 1 log unit in 6 days. In contrast, we found that H37Rv and clinical M. tuberculosis isolates grew significantly more rapidly than H37Ra
in human monocyte-derived macrophages. We used a bacillary inoculum
which was 80-fold lower than that in the study of Paul et al., which
minimized mycobacterial clumping during initial infection and which
more closely mimicked conditions in vivo, where small numbers of
M. tuberculosis cells can establish infection. The low
percentage of infected macrophages minimized decreases in macrophage
viability and ensured an adequate cell population to permit continued
intracellular growth during culture. We observed mean increases in
numbers of CFU of approximately 2 log units with H37Rv and 3 log units
with a clinical isolate. The increased availability of macrophages
relative to bacilli in our experimental system may have facilitated
intracellular growth and enhanced detection of differences in
intracellular growth rates between strains. In addition, Paul et al.
reported that the percentage of infected macrophages did not change
during culture, suggesting that they measured growth within individual
cells but not the spread to adjacent cells. In our study, the
percentage of infected macrophages increased 20- to 50-fold during
culture, indicating that we measured the capacity of M. tuberculosis to grow intracellularly, lyse macrophages, and invade
uninfected cells.
All four M. tuberculosis patient isolates evaluated in
this study proliferated in human macrophages more rapidly than H37Rv, and this difference in proliferation was statistically significant for
isolate ET (Fig. 1). This finding may parallel the increased virulence
of M. tuberculosis strains observed after passage in animals. Additional studies are needed to determine if the growth rates
of patient isolates correlate with disease severity or contagiousness.
The mechanisms underlying the differential growth rates of virulent and
avirulent M. tuberculosis strains in human macrophages remain speculative. H37Ra and H37Rv are similar in their capacities to
enter human macrophages (9), and phagocytosis is mediated through complement receptors. However, only H37Rv utilizes mannose receptors during phagocytosis, and this pathway for cell entry may
influence bacillary intracellular growth rates.
Several monokines influence intracellular mycobacterial
growth in mononuclear phagocytes. TNF- inhibits the intracellular growth of M. tuberculosis in human alveolar macrophages
(5), and IL-10 inhibits the growth of Mycobacterium
avium in murine macrophages (3) but not in human
monocytes (11). IL-12 plays a central role in initiating
effective immunity against mycobacteria (4, 12), although
the direct effects of IL-12 on intracellular mycobacterial growth are
unknown. We found that avirulent and virulent M. tuberculosis strains elicited the production of similar amounts of
TNF-, IL-10, and IL-12, suggesting that these cytokines do not
mediate the differences we observed in intracellular growth rates.
Further studies are needed to characterize the genetic and molecular
mechanisms that control the growth of M. tuberculosis in human macrophages. These studies will improve our understanding of
the virulence of intracellular pathogens and facilitate development of
novel measures to treat and prevent infectious diseases.
| |
ACKNOWLEDGMENTS |
We thank John Belisle for provision of M. tuberculosis H37Ra and H37Rv and Maurice Gately for materials to
measure IL-12 concentrations.
This work was supported by the National Institutes of Health
(AI27285 and AI36069). Mycobacterial products were provided
through contract AI05074 from the National Institute of Allergy and
Infectious Diseases.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Center for
Pulmonary and Infectious Disease Control, The University of Texas
Health Center at Tyler, P.O. Box 2003, Tyler, TX 75710. Phone: (903) 877-5956. Fax: (903) 877-7989. E-mail: pbarnes{at}uthct.edu.
Editor: P. J. Sansonetti
| |
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Infect Immun, February 1998, p. 794-799, Vol. 66, No. 2
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
