 in Patients
with Pulmonary Tuberculosis
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Interferon-
(IFN-) is a cytokine exerting pleiotropic activities, including antimicrobial effects, especially directed against intracellular infectious bacteria. It may be administered by aerosol to reach the
lower respiratory tract without systemic side effects. The aim of the study reported here was the evaluation of aerosolized IFN- treatment (3 MU/dose, given three times a week; total study dose: 72 MU/2 mo) in combination with conventional antimycobacterial therapy in patients with pulmonary
tuberculosis. Two groups of 10 patients each were compared before and after 2 mo of conventional antituberculous chemotherapy with or without inhaled IFN-. Several biologic (bronchoalveolar lavage fluid [BALF] cellularity, Mycobacterium tuberculosis [MT] number in sputum), biochemical (BALF
concentrations of 10 cytokines, BALF IFN- receptor levels), and clinical (fever, vital signs, high-resolution computed tomography [HRCT] images) measures were made in these patients at the time of
their enrollment and at the end of the observation period of the study. Fever, MT number in sputum,
and abnormalities in HRCT images showed significantly earlier resolution in the IFN--treated group,
together with a more significant decrease in BALF interleukin-1
(IL-1), IL-6, and tumor necrosis factor- (TNF-) concentrations and significantly greater pre- versus posttreatment variations in IL-2
and IFN-
. These data, taken together, suggest that IFN- administration may favorably affect the
evolution of pulmonary tuberculosis when combined with antimycobacterial therapy.
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Mycobacterium tuberculosis (MT) causes an estimated 3 million deaths annually worldwide, exceeding those caused by
any other infectious agent (1). Alleviation of the human and
economic costs inflicted by MT requires greater knowledge of
the pathogenesis of tuberculosis. The clinical manifestations
of tuberculosis depend on the cellular immune responses to
the tubercle bacilli, which are characterized by the accumulation of monocytes/macrophages, lymphocytes, and polymorphonuclear leukocytes (PMN) in tuberculous lesions. The immunologic responses are initiated after sensitization of T
lymphocytes by the bacterial antigens of MT, with the release of several cytokines that regulate cell functions. The cellular immune response to MT takes the classic form of delayed-type hypersensitivity that is thought to be mediated by a cooperative interaction between T lymphocytes and macrophages,
depending upon the interplay of cytokines produced by a variety of mononuclear cells including T cells (2). Recent outbreaks of pulmonary tuberculosis underscore the need for
novel approaches to treating and preventing tuberculosis, including the use of immunotherapeutic modalities that enhance normal antimycobacterial defenses. The lung is the only internal organ to which curative or modulating substances can be
applied directly through a natural route so that they can exert
their influence only in the target organ without affecting the
whole organism. Interferon- (IFN-) is a pleiotrophic cytokine with useful infection-control activities; it is produced
primarily by mononuclear phagocytes that are stimulated by
bacteria and viruses, and which exert a wide range of immunomodulatory activities. The availability of pure IFN- preparations permits administration of this modulator by aerosol.
Recent data strongly suggest that IFN- works with interleukin-12 (IL-12) and plays an important role in differentiation
toward the T-helper-cell type 1 (Th1) response, inducing IL-2
and interferon- (IFN-), and inhibiting the T-helper-cell type 2 (Th2) compartment (3). It can now be accepted that IFN-,
released in large amounts by antigen-presenting macrophages,
may favor the production of Th1-like cells by activating the
gene for IFN- in CD4+ T cells and by antagonizing the effect
of IL-4, IL-10, or other immunosuppressive cytokines. Recently, IFN- has been reported to be effective in inhibiting
both antigen (Ag)-induced proliferation and cytokine production by Th2 clones, suggesting that IFN- may favor recovery
in patients with pulmonary tuberculosis (3, 6). Previous
work found that aerosolized IFN- administration to the lung
was well tolerated at biologically active doses. 2'-5' Olygoadenilate synthetase (OAS) levels, used as a marker of IFN- activity, increased after local treatment in serum and bronchoalveolar lavage fluid (BALF), suggesting that the inhaled
cytokine was active at lung level (9, 10).
The aim of the present study was to evaluate the modifications of biologic (sputum MT concentration, cellular spectrum, and numbers of cells in subpopulations in BALF), clinical (fever and high-resolution computed tomographic [HRCT]),
and biochemical (10 cytokines, anti-IFN- antibodies, and
IFN- receptors) variables analyzed in subjects with untreated, active pulmonary tuberculosis observed before and
after 2 mo of therapy consisting of conventional antimycobacterial treatment with or without aerosolized IFN-.
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Study Population
This was an open, parallel study. The study population consisted of 20 human immunodeficiency virus (HIV)-negative patients with newly diagnosed, active pulmonary tuberculosis who presented with a history and chest radiographic findings compatible with pulmonary tuberculosis and who were enrolled in the Chest Clinic of the Lazzaro Spallanzani Institute in Rome. A sputum smear positive for acid-fast bacilli, fever, and loss of weight before admission to the hospital were criteria for inclusion. In addition, all of the patients had positive tuberculin skin tests and no history or signs of any other medical condition requiring current treatment. Bactec (Bactec 460 TB; Becton Dickinson, Milan, Italy) analysis and sputum culture for MT confirmed its presence. Sensitivity tests were adopted to exclude multiresistant strains of MT. Following the results of the susceptibility testing, two patients were excluded from the study because they had drug-resistant strains of MT. All patients were mantained as inpatients, and therapy was administered only by the professional staff.
Patients were randomly subdivided into two groups. Group A (n = 10, comprising six females and four males; three smokers and seven
nonsmokers; mean age = 31 ± 7 yr) was given antituberculous chemotherapy consisting of isoniazid (INH; 5 mg/kg daily), rifampicin (RAMP; 10 mg/kg daily), ethambutol (ETB; 15 to 25 mg/kg daily), and pyrazinamide (PZ; 15 to 30 mg/kg daily). Group B (n = 10, comprising five females and five males; four smokers and six nonsmokers; mean age = 34 ± 13 yr) received a combination of the same antituberculous drugs plus aerosolized human lymphoblastoid IFN- (HuIFN-Ly; 3 MU/dose three times weekly). The dosing schedule was continued for 2 mo. Fever was assessed every day until resolution, and
weight was checked at 1-wk intervals.
Fiberoptic bronchoscopy with bronchoalveolar lavage (BAL) was
performed 24 h after baseline spirometry. The BALF was subjected to
cytologic, analysis and assay for anti-IFN- antibodies and concentrations of several cytokines. From 2 to 4 h after the last dose (total study
dose = 72 MU/2 mo) of HuIFN-Ly, all of the baseline measurements
mentioned previously were repeated. Blood samples were taken from
the patients before and after treatment. Chest radiography and HRCT
were done after 2 mo. None of the patients was given corticosteroids
or other immunosuppressive agents. The study was approved by the
hospital ethics committee, and all subjects gave informed consent.
Safety of Treatment
Patients in Groups A and B were monitored for local and systemic signs and symptoms, and were subjected to routine hematologic blood sampling and blood chemistry and coagulation analyses as well as urinalysis and pulmonary function testing (MasterLab Transfer Spirometer; Jaeger, Würzburg, Germany).
Sputum Induction Protocol and Conversion for MT
Sputum was collected from all subjects. Direct microscopy of smears prepared from sputa after sodium hypochlorite treatment and centrifugation was done every week for 2 mo to evaluate the concentrations of tubercle bacilli. To produce a sputum specimen of sufficient quality and quantity (l to 2 ml), patients inhaled a mixture of nebulized 0.9% hypertonic saline delivered by an Ultraneb 99 Ultrasonic nebulizer (DeVilbiss, Langen, Germany) for 10 min in a total volume of 15 ml of hypertonic saline. Sputum was transferred to a 10 ml screw-cup tube. An equal volume of undiluted sodium hypochlorite (5%) was added and the mixture was incubated at room temperature for 10 min. The tube was shaken regularly. Distilled water was added to fill the tube, and the sample was centrifuged at 3,000 g for 15 min. The sediment was used to prepare smears stained with the Ziehl-Neelsen method. The number of MT was expressed as the mean number MT in 20 fields of view by microscopy (magnification ×40) (11).
HRCT Evaluation
HRCT studies were done with an A-TOM XR 6000 (Ansaldo Elettronica Biomedicale, Genoa, Italy). Sections 1.5-mm thick at 10-mm intervals, with a 512 × 512-pixel reconstruction matrix, instrument settings of 130 kV and 175 mA, and a high-spatial-frequency algorithm were used. All images were obtained at the suspended end-
inspiratory volume with a 1.9-s scanning time. All patients underwent
scanning in the supine position. All images were obtained at window
settings appropriate for lung parenchyma (level = 
400 to 800 HU;
width = 1,800 to 1,600 HU). HRCT scans were evaluated for the presence, distribution, and extent of the following signs of pulmonary tuberculosis: (1) miliary nodules (1- to 2-mm nodules involving both the
intralobular interstitium and interlobular septa); (2) nodules (
10-mm nodules related to the terminal or respiratory bronchioles and
separated from the pleural surface or interlobular septa by more than
2 mm); (3) consolidation (panlobular and polilobular consolidation); (4) a ground-glass appearance; (5) cavitation; (6) bronchial lesions (bronchial wall thickening, bronchiectasis), and (7) fibrotic bands. The
extent of involvement was assessed for each of the three zones of the
lung. On the HRCT scans, the lungs were divided into six zones (upper, middle, and lower zones of the right and left lungs). The upper
zones were defined as areas of the lung above the level of the carina;
the middle zones as areas between the level of the carina and the level
of the inferior pulmonary veins; and the lower zones as areas below
the level of the inferior pulmonary veins. The HRCT score in upper,
middle, and lower lung zones was determined by visually estimating
the extent of disease in each zone (12). Retrospectively, the HRCT
scans were blindly reanalyzed by two independent chest radiologists,
and final conclusions on the findings were reached by means of consensus. The HRCT score was based on the percentage of lung parenchyma that showed evidence of each recorded abnormality. A score of
1 reflected involvement of less than 25% of the image; a score of 2, involvement of 25 to 50%; a score of 3, involvement of 50 to 75%; and a
score of 4, involvement of more than 75%. The scores for each zone
were then added to obtain a global extent score, ranging from 0 to 24, referred to as the HRCT extent score of each HRCT abnormality. A
total score of lung involvement was obtained by summing the global
extent scores of all HRCT abnormalities, ranging from 0 to 192, as an
expression of disease severity.
Processing of BALF
Fiberoptic bronchoscopy was performed before and after antituberculous chemotherapy in all cases. The baseline bronchoscopy was done
within 24 h before the initiation of IFN- treatment. The final bronchoscopy was performed after the last dose of aerosolized IFN-.
Bronchoscopy with BALF collection was done according to a previously described method (13). Prebronchoscopy medications for each
patient included intramuscolar injections of 0.5 mg of atropine; 4%
xylocaine nebulized into the nasopharynx; a total of 4 ml of 1% xylocaine applied directly to the laryngeal area via the bronchoscope,
and 2 ml of 1% xylocaine applied directly to the trachea. The bronchoscope was inserted near a segment of the affected lung with chest
radiographic guidance. A standard lavage protocol was followed by
infusing five aliquots of 20 ml each (a total of 100 ml) of sterile 0.9%
saline, at body temperature, through the aspiration port of the bronchoscope. Lavage fluid was collected via the same port after infusion
of each aliquot by gentle suction into a plastic trap. The fluid recovered was filtered through sterile gauze and the volume was measured.
BALF analysis was performed immediately after bronchoscopy, and
the results were independently verified by a single technician blinded to the patient's condition. The first aliquot was used for counting total
cells with a Burker hemocytometer, and the differential cell analysis
was done by counting 400 cells in smears stained with May-Grunwald-Giemsa. The lymphocyte subpopulation analysis was done flow
cytometrically, using a second aliquot of BALF (with kits purchased
from Becton-Dickinson, Mountain View, CA). The remaining aliquot
was centrifuged at 1,200 × g for 10 min. The cells were washed and resuspended in RPMI (2.5 × 106 cells/ml), and supernatants were frozen
at 80° C until used.
Measurement of Cytokines in BALF
The epithelial lining fluid (ELF) dilution was determined by the urea
method (14) on BALF samples. To determine the urea content of lavage fluid samples, a commercially available kit (Sigma 65 UV; Milan,
Italy) was purchased from Sigma. Cytokine concentrations were measured in supernatants of BALF after 20-fold concentration by means
of Amicon concentrators (Amicon, Beverly, MA). Human IL-1, IL-2,
IL-4, IL-6, IL-8, IL-10, IFN-, and TNF- were measured with an enzyme-linked immunosorbent assay (ELISA; R&D Systems, Minneapolis, MN). Levels of IFN- were measured with a radio immunoassay
(RIA; Nuclear Laser Medicine, Milan, Italy). IL-12 was measured with
an IL-12 + p40 enzyme amplified sensitivity immunoassay (EASIA) kit
(Medgenix Diagnostics, Fleurus, Belgium). Kit sensitivities were as follows: IL-1 = 0.3 pg/ml; IL-2 = 2.5 pg/ml; IL-4 = 4.1 pg/ml; IL-6 = 0.7 pg/ml; IL-8 = 18 pg/ml; IL-10 = 2 pg/ml; IL-12 = 1.5 pg/ml; IFN- = 0.3 pg/ml; IFN- = 3 pg/ml; and TNF- = 4.4 pg/ml.
Expression of IFN- Receptors
An aliquot of BALF cell preparation was incubated at 4° C. The cells
(2.5 to 5 × 105) were added to a final volume of 50 µl/well and washed
by adding 150 µl of phosphate-buffered saline (PBS)/NaN3 to the
wells and centrifuging the cells at 1,000 × g for 3 min. The wash buffer was subsequently aspirated. Cell permeability was obtained by adding
and evaporating methanol (10° C) for 5 min. Cells were again
washed and incubated with 50 µl of anti-IFN- receptor (IFN-R [R-100] antibody; Santa Cruz Biotechnology, Santa Cruz, CA) for 20 min. The optimal antibody concentration was chosen according to the
manufacturer's guidelines. Subsequently, the cells were incubated
with 50 µl of fluoresceinated goat F(ab)2 antirabbit total Ig (Santa
Cruz Biotechnology) for 20 min at 4° C. The cells were washed and
fixed by adding 50 µl of a 2% solution of paraformaldehyde (pH 7.4)
and were incubated at 4° C for 5 min. Following this, the cells were
washed to remove residual paraformaldehyde and unbound fluorescent antibodies. The cells were then analyzed flow cytometrically with
a FACScan cell sorter (Becton Dickinson). The positive fluorescence
intensities were referred to the negative control. For both macrophages and lymphocytes, the results were expressed as relative IFN-R log fluorescence intensity and percentage of IFN-R-positive
cells.
Serum Determination of anti-IFN- Antibodies
Anti-IFN- antibodies were measured with an ELISA (Nuclear Laser
Medicine).
Aerosolized Administration of IFN-
HuIFN-Ly, kindly furnished by Glaxo-Wellcome (Verona, Italy),
was given by an IS-2 jet nebulizer operating on compressed air (Pari,
Starnberg, Germany), generating a total output of 0.32 g/min at an inspiratory flow of 20 L/min, with a delivery time of 4 min and delivery
volume of 1 ml. Particle size analysis was done with a high-resolution
analyzer (Aerosizer Mach2; API, Milan, Italy). Approximately 90%
of the aerosol droplets produced ranged between 0.40 and 3.4 µm
mass median aerodynamic diameter (median = 1.374 µm; standard
geometrical deviation = 1.340 µm [respirable range]). The International Committee on Radiation Protection has fixed a value of 30%
deposition in the lower respiratory tract for droplets this size. Therefore the amounts of IFN- administered were not comparable to
those received. Throughout this report, the administered dose is defined as equivalent to the aerosolized dose.
Statistical Analysis
Owing to the limited number of patients examined, to the lack of knowledge of the data distributions, and to the inevaluability of a number of samples for some of the variables considered, we used a nonparametric statistical analysis. Therefore, the results were expressed as medians and ranges, and comparisons were made by using Wilcoxon's paired rank-sum test for paired measurements or the Mann-Whitney U test for unpaired measurements. To analyze the differences in the data at baseline (T0) and 2 mo (T1) (see Table 1) in both Groups A and B, the T0-T1 differences in the variables were compared, using the Mann-Whitney U test.
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Biological Variables
BALF cellularity. The general characteristics of BALFs are presented in Table 1. The total volume of fluid retrieved, the total number of cells, and the absolute numbers of macrophages and neutrophils per milliliter observed before treatment were not significantly different from those found after therapy in both study groups. By contrast, the lymphocyte counts in Group B were significantly increased after treatment (p = 0.02). No differences were observed as far as the number of lymphocyte alveolitis cases is concerned in the two groups.
The CD4+ and CD8+ T-cell counts were not significantly modified after as compared with before treatment in either study group. Group B, however, showed a significant difference (p = 0.02) in HLA-DR+ T cells after as compared with before treatment. An analysis of the differences (pre- minus posttreatment values) was done for all variables considered. A significant difference was noted only for HLA-DR+ T cells (p = 0.006).
Sputum conversion for MT. The mean numbers of MT bacilli counted in sputum smears (Figure 1a) showed that IFN--treated patients (Group B) had significantly reduced counts
of bacilli at the end of the first week of treatment, whereas the
counts in the group treated only with antituberculous chemotherapy (Group A) changed significantly only at the end of
the second week of therapy. The analysis of the changes for
each patient (pre- minus posttreatment values) showed a significant decrease in numbers of bacilli at the end of the first
week (p = 0.04).
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Clinical Findings
Vital signs. Neither Group A nor Group B showed significant post- versus pretreatment changes in vital signs (blood pressure, heart rate, respiratory rate, and weight; data not shown).
Adverse effects. All patients tolerated the therapy well. No
adverse effects were registered in the group of IFN--treated patients.
Fever. Figure 1b shows that fever in the two groups behaved differently during the first 6 d of treatment. In fact, in evaluating the changes in temperature for each patient (pre- minus posttreatment values), a significant difference was observed in the two groups at the third (p = 0.049) and fourth (p = 0.02) days after the beginning of therapy.
Evolution of HRCT findings. The reversibility of pulmonary damage as a result of 2 mo of treatment was evaluated. In
Group A, the overall disease scores on initial HRCT scans
ranged from 10 to 85 (median = 31), whereas the overall disease scores on follow-up scans ranged from 2 to 72 (median = 24; p = 0.025). In Group B, the overall disease scores on initial
HRCT scans ranged from 16 to 94 (median = 29), whereas on
follow-up scans the overall scores ranged from 7 to 75 (median = 19; p = 0.009). Data for the frequency and extent of HRCT
abnormalities at the first and second evaluations are given in
Table 2 for each HRCT finding. In Group A, a decrease in the
HRCT scores for the frequency and extent of specific abnormalities was found after 2 mo of therapy, but the difference
was not statistically significant. In Group B, in which the patients underwent adjunctive treatment with aerosolized HuIFN-Ly, HRCT abnormalities at the second evaluation showed statistically significant differences from those at the first evaluation for nodules (p = 0.028) and consolidation (p = 0.009) scores.
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Biochemical Variables
Cytokines in BALF supernatants. The release of cytokines into
BALF supernatants from the involved lung segments of tuberculous patients, as measured with ELISA, is shown in Table 3.
After 2 mo of treatment, none of the cytokines assigned
reached levels statistically significantly different from the levels observed before treatment, with the exception of TNF-
and IL-6 in both Groups A and B; IL-1 was significantly decreased only in Group B. However, it is important to note that
the differences were more significant in Group B (Table 3).
When the T0-T1 changes were compared in Groups A versus
B, TNF- and IL-6 were still significantly different. New findings were significant differences for IL-2 and IFN-. Their behavior was consistent with that of the CD4/CD8 T-cell ratio
shown in Table 1.
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IFN- receptor levels. Figure 2 shows IFN-R expression as
evaluated flow cytometrically in BALF cells of Groups A and
B before and after treatment. In Group A, lymphocytes evaluated after therapy had a median log fluorescence intensity not
different from that before therapy (with 85% of the cells
showing specific IFN-R positivity before and 77% after therapy). Before therapy in Group B, the lymphocytes had a median log fluorescence intensity significantly lower than that
observed after therapy (p = 0.01) (the number of cells showing specific IFN-R positivity rose from 73% to 75%).
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In Group A, macrophages showed a median IFN-R log
fluorescence intensity that did not change statistically from
before to after treatment. Before treatment, 94% of the cells
showed specific IFN-R positivity, which increased to 97%
after treatment. The same results were observed for macrophages in Group B (with 93% of the cells showing specific
IFN-R positivity before therapy and 91% after therapy).
Serum determinations of anti-IFN- antibodies. The assay
for anti-IFN- antibodies was negative in all patients, before
and after 2 mo of treatment (data not shown).
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Pulmonary tuberculosis is an infectious disease caused by MT,
a very resistant microorganism with intracellular localization. At present, antimycobacterial therapy includes a panel
of combined antibiotics intended to provide maximum efficacy
and rapidity of disease resolution and limitation of side effects. Despite this massive therapeutic approach, treatment
must be continued for a long time (at least 6 mo) to avoid frequent relapses caused by failure to eradicate the microorganism in the short term (15). Any therapeutic approach that would
enhance natural host defenses would clearly be important once
its efficacy was established. Different immunomodulatory substances have been reported as capable of controlling the infection with MT. Generally, these substances belong to the group
of cytokines, especially IL-2, IL-12, IFN-, and TNF-. These
molecules exert their effects by activating different types of
cells involved in microorganism clearance (16). Another cytokine molecule, IFN-, has recently been reported to be
capable of controlling MT (20). However, this cytokine produces toxicity, and we therefore decided to instead explore the
effects of IFN-, which is less expensive and has been more extensively studied in humans (21, 22).
Originally considered a simple antiviral substance, IFN-
has since been shown to exhibit a variety of biologic effects.
Early studies reported multiple effects of IFN- on the immune response in vitro as well as in vivo, including effects on
antibody production, natural killer (NK) cell activity, antigen
presentation, and phagocytosis (23). More recently, IFN- has
been shown to regulate T-cell function and to particularly
stimulate the Th1 subset. In contrast, it inhibited both antigen-induced proliferation and cytokine production by Th2 clones
(6). Consequently, IFN- can increase the IFN--producing CD4+ population of T-cells and antagonize the suppressing effects of IL-4 (3). In mice, cytokine production (such as IL-2
and IFN-) by Th1 cells is associated with protection against
tuberculosis, whereas Th2-produced cytokines are associated
with increased susceptibility to the disease (24, 25). Furthermore, animal and in vivo studies also show that progressive
tuberculosis is associated with a Th2 response, whereas regression of the infection is characterized by enhancement of
the Th1 compartment and release of Th1-produced cytokines
(26). Therefore, one of the aims of the present study was to
evaluate the effect of IFN- administration in combination with
conventional chemotherapy in patients with pulmonary tuberculosis.
To avoid the side effects already described for IFN-, we followed the direction provided by a previous study done by our group (10) and decided to treat patients with IFN- given by aerosol. As previously shown, this cytokine can be safely delivered to the epithelial surface of the lower respiratory tract
without systemic side effects (10). To establish possible mechanisms involved in infection control by IFN-, we evaluated several biologic, clinical, and biochemical variables. Among these
variables we found that the number of MT in sputum and the
pattern of cells in BALF were significantly modified when
pre- and posttreatment determinations were compared (Figure 1 and Table 1). In fact, sputum microscopic conversion
was clearly anticipated by a week after the beginning of treatment in patients receiving the combination therapy including
IFN-. Since different cell types (such as monocytes/macrophages, T lymphocytes, and neutrophils) are considered important mediators of bacterial clearance, we analyzed BALF cells
both qualitatively and quantitatively by means of flow cytometric techniques. Pretreatment findings in the patients on
whom this was done were consistent with those reported in
the literature, with increased numbers of lymphocytes and
granulocytes, as well as decreased numbers of monocytes (27).
When we made a comparison of flow cytometric results before
and after 2 mo of therapy in our study Groups A and B, only
Group B, receiving IFN-, showed significant increases in total
lymphocytes and HLA DR+ cells. The total lymphocyte increase agrees with the known protective effect of CD4+ T cells
against Mycobacterium avium in mice (28). Besides evaluating biologic variables, we evaluated two clinical aspects of tuberculosis: fever and radiologic features. Corresponding to MT
reduction in sputa, fever also decreased more rapidly in patients receiving IFN-. This is a second important indication
that combination therapy including IFN- may have a rational
role in treating tuberculosis.
The third crucial indicator used to follow the evolution of
pulmonary tuberculosis was HRCT. More sensitive than chest
radiography for the detection and characterization of subtle
parenchymal disease, HRCT may also be of value in detecting
and following diffuse lung involvement (when corresponding
chest radiographs are normal), or in showing minimal or limited disease (29). In our study, HRCT permitted the evaluation
of some of the specific variables (listed in Table 2) that can describe the evolution of tuberculosis (30). These include two
abnormalities: nodules and areas of consolidation. HRCT
scores represent both the most important variables of activity
for pulmonary tuberculosis and those variables showing the
most rapid variations over time. Therefore, the significant reduction in scores for these variables, observed only in IFN--treated patients, could corroborate the utility of IFN- treatment. As far as biochemical variables are concerned, several
determinations were done. As is known, cytokine receptors are
generally induced by the same molecule they bind (31), and
their increase therefore represents a marker of cytokine activity. Since the treatment in one arm of our study was based on
combination therapy including IFN-, we analyzed IFN- receptors both on lymphocytes and on monocytes/macrophages
from BALF. The data showed that IFN- receptors expressed
on BALF lymphocytes of patients receiving IFN- were increased concomitantly with disease improvement. In the same period, measurements of three cytokines showed significant
decreases from before to after 2 mo of therapy. In particular,
levels of IL-1, IL-6, and TNF- dropped in BALF after treatment.
It was also noted that in patients not given IFN-, the same
cytokines also fell to lower levels than before treatment, although significant differences were observed only for IL-6 and
TNF-. Furthermore, the significance of the cytokine variations
was greater in IFN--treated than in non-IFN--treated patients. This suggests that changes in proinflammatory cytokines,
possibly linked to the reduction of inflammatory phenomena,
are associated with disease improvement in tuberculosis. It is
not surprising that the three cytokines named here, IL-1, IL-6,
and TNF-, exhibited behavior according with this finding.
These three cytokines act synergistically, and their amounts
often correlate in different diseases. A more sensitive comparison of the T0-T1 (see Table 3) changes observed for the different cytokines in Groups A and B revealed possibly important differences in IL-2 and IFN-. Literature data show that
TNF-, IFN-, and IL-2 can exert antimycobacterial activity (18, 32). The approach used in our study did not permit a specific analysis of which kind of cells produced these mediators, although it is reported in the literature that a wide spectrum of
cells can release them, especially activated monocytes/macrophages and T lymphocytes. Our findings did not reflect increases of IFN- in IFN--treated patients, possibily because
of the short, 2-mo posttreatment observation time, during
which both the effect of IFN- and disease recovery were effective. A particular point of note is the methodology we used for
determining and expressing cytokine levels. In our study, cytokine concentrations were normalized by the dilution factor
determined by the volume of the saline injection used to obtain BALF (14). The few data reported in the literature on this
topic generally show BALF cell cytokine release, making
comparisons with our results impossible (33). In addition,
no data are available on comparisons of cytokine concentrations analyzed before and after therapy.
In conclusion, even though the data discussed do not clarify
the mechanisms involved, the patients receiving conventional chemotherapy plus IFN- in our study showed more favorable
effects than those given chemotherapy alone. The data presented here, if confirmed with a greater number of subjects,
open a wide spectrum of possibilities, including that of using
aerosolized IFN- in both HIV-negative and HIV-positive tuberculosis patients to enhance their natural response against
MT. Specific trials must be planned to explore the best schedule and doses for such treatment, and the possibility that
IFN- favors the clinical outcome in patients infected with
multiresistant strains of MT also needs to be evaluated, as
does the possibility that shorter periods of conventional therapy may be established to limit side effects. In addition, experiments in vitro and in animal models are needed to analyze the
possible mechanisms involved in the effects of treating tuberculosis with IFN-.
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Footnotes |
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Correspondence and requests for reprints should be addressed to Dr. Sandro Giosuè, Istituto Lazzaro Spallanzani, IRCCS, Clinica Malattie dell'Apparato Respiratorio, Via Portuense 292, 00149 Rome, Italy. E-mail: Giosue{at}LINET.IT
(Received in original form March 16, 1998 and in revised form June 9, 1998).
Acknowledgments: The authors gratefully acknowledge Prof. C. Saltini for his helpful comments and suggestions, Prof. G. Manfredi for statistical analysis, and S. Watson for preparation of the manuscript.
Supported in part by grant 95.02145.04 from the Consiglio Nazionale delle Ricerche.
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References |
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INTRODUCTION
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REFERENCES
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1. Murray, C. J. L., K. Styblo, and A. Rouillon. 1990. Tuberculosis in developing countries: burden, intervention and cost. Bull. Int. Union Tuberc. Lung Dis. 65: 6-26 [Medline].
2. Edwards, D., and C. H. Kirkpatric. 1986. The immunology of mycobacterial diseases. Am. Rev. Respir. Dis. 134: 1062-1071 [Medline].
3.
Brinkmann, V.,
T. Geiger,
S. Alkan, and
C. H. Heusser.
1993.
Interferon
alpha increases the frequency of interferon gamma-producing human
CD4+ T cells.
J. Exp. Med.
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