|
||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
 |
ABSTRACT |
|---|
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
We have investigated both modifications in natural (innate) immunity caused by chronic obstructive pulmonary disease (COPD) and the effects of a glycophosphopeptical immunomodulator (Inmunoferón) treatment on COPD-associated immunoalterations. In
a double-blinded clinical trial, 60 patients with COPD received glycophosphopeptical or placebo during 90 consecutive days at oral
doses of 3 g/d. Fifty-six sex- and age-matched healthy control subjects were included as a reference group for immunologic parameters. Peripheral blood natural killer (PBNK) cell cytotoxic activity
and phagocytic activity of peripheral monocytes/macrophages
(Mo/Ma) and polymorphonuclear (PMN) cells were assessed at
baseline and then again at the end of treatments. We found both
PBNK activity and phagocytic activity to be significantly decreased
in patients with COPD compared with levels in healthy volunteers.
The treatment with glycophosphopeptical provoked significant
stimulatory effects on PBNK cytotoxic activity. This stimulation
was not mediated by an increase in CD3
CD56+ NK cells. Further,
glycophosphopeptical significantly increased the percentage of
monocytes and PMNs that phagocytize Escherichia coli in vitro, as
well as increased phagocytic indices. We conclude that peripheral
blood cells of patients with COPD show clear defects in natural immunity that are partially rescued by glycophosphopeptical.
| |
INTRODUCTION |
|---|
|
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
Chronic obstructive pulmonary disease (COPD) is a clinically defined respiratory disease with a high prevalence worldwide (1). Although the intrinsic mechanisms involved in the pathogenesis of COPD are partially unknown, it has been shown that COPD is frequently associated with several immune disturbances. Abnormalities in the distribution and in the function of T-lymphocyte (2) and natural killer (NK) cell (6) subsets in patients with COPD have been documented in the literature. Alterations in effector functions and cytokine production by monocytes and polymorphonuclear cells (PMNs) have been described in patients with COPD (7). The pathophysiology of these immune alterations is complex. Several contributory factors may be involved in this immunologic impairment, including cigarette smoking (5, 15), age (18), and relapsing viral and bacterial respiratory infections (1, 7, 10). Of the aforementioned factors, the contribution of smoking to observed immunodeficiencies in COPD has proved the most controversial.
The pathogenic relevance of the impairment of phagocytic cells and NK lymphocytes in patients with COPD is unclear. Although patients with defects in NK (19) or phagocytosis activity (20, 21) are highly susceptible to viral or bacterial infections, the relative contribution of these impairments to the increased prevalence of acute respiratory infections in patients with COPD (1, 6, 10) has yet to be established. Epidemiologic studies have implicated recurrence of acute respiratory infections as one of the major factors associated with the progression of chronic airway obstruction (1, 22). In patients with COPD, superimposed acute respiratory infections result in clinical relapses. The argument for the use of immunomodulators in patients with COPD is well supported by clinical evidence of reduced recurrence rates of acute respiratory infections (23).
Glycophosphopeptical is an immunomodulator that has
been proven to increase NK and some macrophage activities
in human and animal models (18, 27). In animal models, the
capacity of glycophosphopeptical to potentiate natural (innate) and specific immunity is related to the induction of endogenous production of interleukin-12 (IL-12) and interferon
gamma (IFN-
) while partially inhibiting the production of tumor necrosis factor-alpha (TNF-
) (28, 29). Glycophosphopeptical potentiates the in vitro immune response against
some viruses (30) and viral vaccines (31), demonstrating the
potential in vivo immunologically mediated antiviral activity
of the drug. Whereas the efficacy of glycophosphopeptical in
protecting patients with COPD from acute infectious exacerbations is well established (23), the mechanism of its ability
to rescue immunoalterations in humans remains undefined.
Because observed changes in natural immunity in COPD may
contribute to increased risk of infectious complications, we investigated the effect of glycophosphopeptical on peripheral
blood natural killer (PBNK) activity and monocytes/macrophages (Mo/Ma) and PMN phagocyte activity in a large population of COPD patients in a randomized, placebo-controlled, double-blind clinical trial. We also included sex- and age-matched healthy control subjects as a reference group against
which to compare the ability of glycophosphopeptical to reverse immunoalterations seen in patients with COPD.
| |
METHODS |
|---|
|
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
Inclusion and Exclusion Criteria
Subjects of the study were individuals of both sexes between the ages of 40 and 80 with a diagnosis of COPD as defined by the American Thoracic Society guidelines (32) and a Karnofsky score greater than 70.*
Inclusion criteria. Diagnosis of COPD was defined by the following spirometry parameters: FEV1/FVC < 70% and FEV between 35 and 70% with no evidence of a significant reversible component as evidenced by a less than 15% (200 ml) change from baseline after bronchodilator challenge. At least two episodes of acute respiratory exacerbations during the previous year were required for inclusion into the study. Respiratory exacerbations were defined as having at least one of the following: worsening productive cough, increasing production of purulent sputum, increasing dyspnea, or pneumonia. Further, subjects must have had a history of smoking at least one pack a day for 20 yr and have quit smoking at least 6 mo before study inclusion.
Exclusion criteria. Subjects unable or unlikely to comply with the study protocol (e.g., drug or alcohol dependence) were excluded. Female subjects were excluded in the case of pregnancy, breast feeding, or refusal to use a standard birth control method. Subjects with previously identified allergies to Inmunoferón (glycophosphopeptical) or one of its components were excluded.
Subjects with congenital or acquired immunodeficiencies or autoimmune disease were also excluded. In addition, subjects with the following diagnoses were excluded: malabsorption syndrome, hypercalcemia, bronchiectasis, active pulmonary tuberculosis, pulmonary or extrapulmonary neoplasm, cystic fibrosis, restrictive pulmonary fibrosis, cardiac insufficiency greater than or equal to class III; advanced renal insufficiency (serum creatinine > 4 mg/dl) or liver disease with a Child-Pugh score of 7 to 15 (Grade B or C).
Subjects who in the 3 mo before the study received immunosuppressants, immunomodulators, cimetidine, or other medications considered to modify the immune response except inhaled corticosteroids (maximum dose of 800 µg of beclomethasone or equivalent dosing of other inhaled corticosteroids) and subjects who received systemic corticosteroid therapy within 2 wk before entrance into the study were excluded. Further, any subjects who experienced an acute respiratory exacerbation treated with antibiotics within the month before the study and those with a clinical destabilization within 15 d of the study were not included.
Subjects
In a double-blind clinical trial 60 patients with COPD as defined previously were randomized to receive glycophosphopeptical (n = 30) or an indistinguishable placebo (n = 30). Subject characteristics are shown in Table 1. Before study entry, all recruited subjects received extensive information about the study, were given the opportunity to ask questions, and signed a witnessed informed consent. An age- and sex-matched control group of 56 healthy, nonsmoking donors with a mean age of 61 ± 8 yr was used for the immunologic studies. The study was approved by the Research and Ethics Committee of Alcalá University.
|
The study began in September 1998, before the onset of winter in Spain. Peripheral venous blood was collected from all patients with COPD and healthy volunteers to assess baseline immunologic parameters. Sixty patients with COPD received either glycophosphopeptical or placebo during 90 consecutive days during the winter months. Peripheral blood for final measurements of immunologic parameters was collected again within 6 d of terminating treatment. The total number of subjects reported for any given experiment reflects the number of subjects available for the given analysis. Four patients in the placebo group were lost to follow-up. No deaths occurred during the study period. Any discrepancy between the enrolled patients and final subject number reflects either patient dropout or insufficient sample to perform the experiment.
Treatments
Glycophosphopeptical (AM3 Inmunoferón; I. F. Cantabria, Madrid, Spain) is an orally given immunomodulator with a low toxicity profile that is a polysaccharide/protein compound purified from Candida utilis. Previous dose-finding and kinetic studies with glycophosphopeptical demonstrated that 3 g/d was the optimal dose for maximal immunostimulation without side effects (25). Six capsules per day (two 500-mg capsules three times a day) of either glycophosphopeptical or placebo were therefore administered orally during 90 consecutive days.
Cell Separation
Peripheral blood mononuclear cells (PBMCs) were obtained by Ficoll-Hypaque (Lymphoprep Nyegaard and Co., Oslo, Norway) density gradient centrifugation, washed three times in NaCl 0.9% buffer, and suspended in RPMI 1640 (Whitaker Bioproducts, Walkerville, MI) containing 10% fetal bovine serum (Biochrom KG, Berlin). After counting, cells were resuspended at 1 × 106 cells/ml in RPMI 1640 supplemented with 10% heat-activated fetal bovine serum, L-glutamine (2 mM Flow Laboratories, Irvine, UK), Hepes (0.5% Flow Lab) and 1% penicillin-streptomycin (Difco Laboratories, Detroit, MI); this will be referred to as complete medium. Cell viability was checked by trypan blue exclusion.
Cytotoxicity Assays
Cytotoxicity was quantified by a 51Cr-specific release assay using K-562
target cells, as previously described (26). Target cells were labeled
with Na251CrO4, washed twice, and resuspended in culture medium.
Target cells (5 × 104 cells/ml) were mixed with effector cells at different effector to target (E/T) ratios (50:1, 25:1, 12:1, and 6:1) in triplicate round-bottom microwell plates (Soria-Greiner, Madrid, Spain). Controls included target cells incubated either with complete medium
(spontaneous 51Cr release) or with 1 N HCl (maximal 51Cr release).
Plates were incubated for 4 h at 37° C in a 5% CO2 humid atmosphere. After incubation, 0.1 ml from each well was collected and
counted in a gamma counter. All cultures were made in triplicate and
mean counts per minute (cpm) used for all calculations. The percentages of specific lysis were calculated as follows: (A
S / MS) × 100, where A = mean cpm of test samples, S = mean cpm of spontaneous
51Cr release, and T = mean cpm of maximal 51Cr release. Spontaneous
51Cr release was always lower than 15% of maximal release counts.
Immunophenotypic Studies
PBMCs (5 × 105 in 50 µl of phosphate-buffered saline [PBS] with 2% human albumin) were incubated with combinations of fluorescein isothiocyanate (FITC), phycoerythrin (PE), and phycoerythrin-cyanine-5 conjugate (tricolor)-labeled monoclonal antibodies (MoAbs) against CD3, CD14, CD15, CD16, and CD56, for 30 min at 4° C as previously described (33, 34). Isotype-matched irrelevant FITC-, PE-, and tricolor-labeled MoAbs served as a control for each experiment. After washing cells three times in PBS, individual cell fluorescence was measured and registered with a FACScan (Becton-Dickinson, San Jose CA). Flow cytometric analysis was completed with the help of Cell Quest software (Becton Dickinson).
Flow Cytometry Studies on Phagocytic Activity
Each assay was performed in duplicate with 100 µl of cold heparinized whole blood according to methods previously described using Phagotest (ORPEGEN Pharma, Heidelberg, Germany) (35). In brief, after the addition of 20 × 106 FITC-labeled opsonized Escherichia coli (Becton Dickinson) the samples were incubated for 10 min at 37° C. To suppress the fluorescence of bacteria attached to the outside of the cells, 100 µl of ice-cold quenching solution (trypan blue) was added to the samples before washing and pelleting (2 times at 250 g × 5 min). Samples were then treated with FACS lysing solution (Becton Dickinson) that lyses red cells while fixing leukocytes. Negative control samples were treated as above with the exception of the initial incubation step, which included cells alone or with E. coli incubated on ice; and cells alone incubated at 37° C. Staining with propidium iodide allowed for identification of leukocytes. Fluorescence was analyzed with a FACScan (Becton-Dickinson, San Jose CA) Both the percentage of monocytes and PMN phagocytes with phagocytized bacteria and the mean phagocytic activity per phagocytic cell (mean channel intensity) were determined. The total phagocytic activity (phagocytic indices) of the population was determined by multiplying the percentage of phagocytic cells by the mean phagocytic capacity per cell.
Statistical Analysis
Differences between groups were compared for normally distributed
data by two-tailed Student's t test. Comparisons of pretreatment and
posttreatment immunologic parameters within groups were completed by paired t-test. Significance was set at p 
0.05.
| |
RESULTS |
|---|
|
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
Decreased Circulating NK Activity in Patients with COPD Is Rescued by Glycophosphopeptical Treatment
The NK activity of PBMCs from patients with COPD was investigated before randomization (baseline) and then again after the end of glycophosphopeptical treatment. As shown in Table 2, patients with COPD showed significantly lower baseline PBNK cell activity at all E/T ratios than did age-matched healthy control subjects. Further, at baseline values there were no significant differences between the PBNK activity in glycophosphopeptical or placebo treatment groups of COPD patients (Table 2). At follow-up we show no significant change in PBNK cell activity in the placebo group (Figure 1A). In contrast, glycophosphopeptical treatment significantly increased PBNK activity from baseline at all E/T ratios analyzed (Figure 1B). Glycophosphopeptical treatment increased PBNK activity to such a degree that it reached the level of healthy control subjects as measured at follow-up (Figure 2). However, the PBNK activity in the placebo group continued to be significantly depressed as compared with healthy control subjects at the time of follow-up (Figure 2).
|
|
|
The increase in PBNK activity in the glycophosphopeptical-treated COPD patient group was not the result of an increase in NK cell number. The percentage of CD3CD16+ or
CD3CD56+ NK cells in patients with COPD and in healthy
control subjects did not differ significantly at baseline or at
follow-up (data not shown). Neither did we find significant
changes in the percentages of NK cells from baseline to follow-up in patients with COPD (glycophosphopeptical [baseline 19.2 ± 14.1; follow-up 22.7 ± 7.6] nor placebo [baseline 25.6 ± 16.2; follow-up 29.2 ± 13.5] groups).
Glycophosphopeptical Treatment Rescues Percentage of Circulating Phagocytic Cells and Phagocytic Activity Per Cell in Patients with COPD
Tables 345 show the percentage of phagocytic cells, mean phagocytic activity per cell, and phagocytic indices for each cell type as measured in patients with COPD and healthy control subjects at baseline and follow-up. Patients with COPD had significantly depressed phagocytic activities of monocytes and PMNs compared with levels observed in healthy volunteers (Table 3). Whereas the three baseline parameters of phagocytic activity of both monocytes and PMNs in the COPD group were significantly decreased with respect to that of healthy donors, glycophosphopeptical treatment, but not placebo, normalized these responses at posttreatment follow-up.
|
|
|
At baseline the patients with COPD in the glycophosphopeptical and placebo treatment groups did not significantly differ in phagocytic activity of peripheral blood monocytes (Table 4) or PMNs (Table 5). Glycophosphopeptical treatment significantly increased both the percentage of phagocytic cells in PB monocytes (Table 4) and PMNs (Table 5) and the phagocytic indices of monocytes (Table 4) and PMNs (Table 5). Although the mean phagocytic capacity per individual cell trended upward after glycophosphopeptical treatment in both monocytes (Table 4) and PMNs (Table 5), the increases did not reach statistical significance. Patients with COPD in the placebo-treated group did not demonstrate any significant changes at follow-up in any of the three parameters of the PB monocyte (Table 4) or PMN (Table 5) phagocytic activity.
To investigate whether the differences in active phagocytic cell number reflected differences in monocyte or PMN phagocytes, phenotypic analysis was done for CD14 and CD15 in healthy and COPD patients (glycophosphopeptical and placebo groups). There were no significant differences in the percentage of monocytes (CD14bright CD15dim) or PMN phagocytes (CD14dim CD15bright) within any of the study groups either at baseline or at follow-up (data not shown). Further, glycophosphopeptical or placebo treatment did not significantly alter the percentage of PMNs or monocytes (data not shown).
| |
DISCUSSION |
|---|
|
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
The presence and relevance of immunoalterations in COPD have been repeatedly challenged. This study did not attempt to define whether immunoalterations were caused directly by COPD pathophysiology. However, this report clearly demonstrates that patients with COPD have decreased PBNK cytotoxic activity and impaired monocytes and PMN phagocytic activities when compared with age-matched healthy control subjects. Although alterations in NK cell activity in COPD have been correlated with tobacco consumption (8, 15, 36), no prior study has been done that consistently demonstrates a direct effect of COPD in the absence of active smoking. Because we excluded active smokers from this study, the defective PBNK activity seen in patients with COPD cannot be explained by active tobacco use alone. Much of the controversial data about COPD-mediated alterations in innate and specific immunity can likely be accounted for by the fact that the onset of COPD and its clinical evolution are influenced by multiple factors such as genetics, tobacco, infectious exacerbations, seasonal variations, and patient age. Treatment with glycophosphopeptical restores PBNK activity to the level of healthy control subjects despite the multifactorial origin of declines in PBNK activity among patients with COPD.
Together with NK cells, the Mo/Ma system as well as PMNs play a pivotal role in innate immunity. Functional alterations in Mo/Ma and PMNs have been described in many human infectious diseases, but also in patients with increased predisposition for developing respiratory infections such as COPD (1, 7, 10, 11, 18, 37). In this study we have demonstrated that patients with COPD show defects in phagocytic functions of Mo (Table 4) and PMNs (Table 5).
A novel finding of this study is that glycophosphopeptical treatment returns monocyte phagocytic activity in patients with COPD to the level seen in healthy control subjects (Table 4). Although it has been previously demonstrated that glycophosphopeptical enhances the capacity of purified monocytes to phagocyte Candida albicans (25), the sensitivity of this finding was limited by the microscopic technique. In contrast, our flow cytometry method allowed the quantification of the phagocytic activity of a high number of individual cells (n = 10,000), several folds larger than that determined by microscopic observation (n = 300), thus improving the accuracy of the quantification of phagocytic activity. Because of the enhanced sensitivity of this method, we were able to demonstrate that the stimulatory effect of glycophosphopeptical upon the phagocytic activity of monocytes and PMNs is mainly due to an increase in the percentage of cells with phagocytic capacity, although it also reflects an increase in phagocytic capacity per cell. These data, together with the high degree of monocyte activation reported by other investigators (18, 27), and the high degree of monocyte stimulation observed herein (Table 4), clearly suggest the Mo/Ma system is the primary target for the immunologic actions displayed by glycophosphopeptical.
The decline in PMN phagocytic activity in patients with COPD is well established (6, 11, 38). Furthermore, similar studies of flow cytometry have demonstrated comparable findings of diminished phagocytosis and killing of nonencapsulated Haemophilus influenzae by PMNs (39). Our finding that glycophosphopeptical increases the phagocytic activity of PMNs (Table 5) is biologically important because PMNs far outnumber monocytes in peripheral blood and thus are the most frequently found phagocytic cells in the human body.
In conclusion, our use of a large, ex-smoker patient population allows us to show clear deficiencies in natural immune mechanisms such as PBNK cytotoxic activity and phagocytosis of peripheral blood monocytes and PMNs in COPD that cannot be accounted for by active smoking alone. These data in this selected population of COPD patients with a history of a high incidence of recurrent acute respiratory exacerbations (probable infectious origin) further support the possible clinical relevance of the demonstrated COPD-related alterations in natural immunity as a pathway to the development of infectious complications. Further, these alterations are fully rescued by glycophosphopeptical treatment. Given the importance of innate immunity against microbial invasion, it is likely that the defects in NK and PMN/monocyte phagocyte activity are, at least in part, responsible for the high rate of infectious exacerbations seen in patients with COPD. Antimicrobial management of patients with COPD is becoming increasingly difficult with the continued emergence of antibiotic resistance and the presence of multiple strains of H. influenzae with different antimicrobial susceptibility profiles (40) in the sputum of patients with COPD. Thus the use of immunomodulators offers a great advantage in the successful management of these patients. The next step is to test the clinical efficacy of the immunostimulant effects of glycophosphopeptical on NK and PMN/monocyte phagocytic activity in patients with COPD. We are currently enrolling patients in a multicenter double-blind clinical trial in order to evaluate the relationship between immune parameters and rates of superimposed respiratory infections in patients with COPD.
| |
Footnotes |
|---|
Correspondence and requests for reprints should be addressed to Melchor Alvarez-Mon, M.D., Ph.D., Professor and Chair, Department of Medicine, University Hospital "Príncipe de Asturias," Alcalá University, Carretera Madrid-Barcelona, Km 33,600, 28871 Alcalá de Henares, Madrid, Spain. E-mail: mams{at}tsai.es
(Received in original form February 4, 2000 and in revised form October 29, 2000).
This work was partially supported by grants from Comisión Interministerial de Ciencia y Tecnología (Plan Nacional de Salud) and Feder RFD 1997-1950, Spain.Alfredo Prieto and Eduardo Reyes are joint first authors.
* The Karnofsky Rating Scale is a scale of disability where 100 is "Normal with no complaints or evidence of disease," 90 is "Able to carry on normal activity but with minor signs of illness present," 80 is "Normal activity but requiring effort with signs and symptoms of disease more prominent," 70 is "Able to care for self, but unable to work or carry on other normal activities," 60 is "Able to care for most needs, but requires occasional assistance," 50 is "Considerable assistance and frequent medical care required; some self-care possible," 40 is "Disabled, requiring special care and assistance," 30 is "Severely disabled; hospitalization required but death not imminent," 20 is "Extremely ill; supportive treatment and/ or hospitalization required," 10 is "Imminent death," and 0 is "Death."
Acknowledgments:
The authors thank the efforts of the Group of Research
of the Immune System Involvement in Respiratory Diseases (C. Garcia Calvo, M.D., Ph.D. [Department of Medicine, I. F. Cantabria, Madrid]; J. Jareño,
M.D. [Hospital Del Aire, Madrid]; J. M. Rodriguez, M.D. [Hospital Universitario Gregorio Marañon, Madrid]; M. Calle, M.D. [Hospital Universitario
Clinico San Carlos, Madrid]; E. Sauz and A. de la Hera [Department of Medicine, University of Alcalá]) in developing the study protocol and recruiting
patients for inclusion.
| |
References |
|---|
|
TOP
ABSTRACT
INTRODUCTION
METHODS
RESULTS
DISCUSSION
REFERENCES
|
|---|
1. Reynolds HY. Chronic bronchitis and acute infectious exacerbations. In: Douglas RJ Jr, Bennett JE, and Mandell GL, editors. Principles and practice of infectious diseases, 3rd ed. New York: Churchill Livingstone; 1990. p. 531-535.
2. O'Shaughnessy TC, Ansari TW, Barnes NC, Jeffery PK. Inflammation in bronchial biopsies of subjects with chronic bronchitis: inverse relationship of CD8+ T lymphocytes with FEV1. Am J Respir Crit Care Med 1997; 155: 852-857 [Abstract].
3. Jansen HM, Sachs AP, van Alphen L. Predisposing conditions to bacterial infections in chronic obstructive pulmonary disease. Am J Respir Crit Care Med 1995; 151: 2073-2080 [Abstract].
4. Baglioni S, Dottorini M, Sini GM, Eslami A, Vecchiarelli A, Todisco T. Prediction of pulmonary immunodeficiency in chronic bronchitis by cutaneous hypoergy to multitest. Dev Biol Stand 1992; 77: 167-173 [Medline].
5. Qvarfordt I, Riise GC, Larsson S, Almqvist G, Rollof J. Cutaneous delayed-type hypersensitivity reactions in smokers with chronic bronchitis and recurrent exacerbations: comparison with asymptomatic smokers and never-smokers. Respir Med 1999; 93: 491-497 [Medline].
6. Fietta A, Bersani C, De Rose V, Grassi FA, Mangiarotti P, Uccelli M, Grassi C. Evaluation of systemic host defense mechanisms in chronic bronchitis. Respiration 1988; 53: 37-43 [Medline].
7.
Qvarfordt I,
Riise GC,
Larsson S,
Almqvist G,
Rollof J,
Bengtsson T,
Andersson BA.
Immunological findings in blood and bronchoalveolar
lavage fluid in chronic bronchitis patients with recurrent infectious exacerbations.
Eur Respir J
1998;
11:
46-54
8. Costabel U, Maier K, Teschler H, Wang YM. Local immune components in chronic obstructive pulmonary disease. Respiration 1992;59 (Suppl 1):17-19.
9. Chanez P, Enander I, Jones I, Godard P, Bousquet J. Interleukin 8 in bronchoalveolar lavage of asthmatic and chronic bronchitis patients. Int Archives Allergy Immunol 1996; 111: 83-88 .
10. Nielsen H, Bonde J. Immunostimulation of blood monocyte function by RU 41.740 (Biostim) in patients with chronic bronchitis. Int J Immunopharmacol 1986; 8: 589-592 [Medline].
11. Venge P, Rak S, Steinholtz L, Hakansson L, Lindblad G. Neutrophil function in chronic bronchitis. Eur Respir J 1991; 4: 536-543 [Abstract].
12. Nielson H. Inflammatory indices in chronic bronchitis: monocyte- macrophage microbicidal activity. Agents Actions 1990;30(Suppl): 213-218.
13. Martin TR, Raghu G, Maunder RJ, Springmeyer SC. The effects of chronic bronchitis and chronic air-flow obstruction on lung cell populations recovered by bronchoalveolar lavage. Am Rev Respir Dis 1985; 132: 254-260 [Medline].
14. McCusker KT, Hoidal J. Leukocyte function and chronic bronchitis. Semin Respir Infect 1988; 3: 5-13 [Medline].
15. Phillips B, Marshall ME, Brown S, Thompson JS. Effect of smoking on human natural killer cell activity. Cancer 1985; 56: 2789-2792 [Medline].
16. Holt PG. Immune and inflammatory function in cigarette smokers. Thorax 1987; 42: 241-249 [Medline].
17. Lusuardi M, Capelli A, Cerutti CG, Spada EL, Donner CF. Airways inflammation in subjects with chronic bronchitis who have never smoked. Thorax 1994; 49: 1211-1216 [Abstract].
18. Villarrubia VG, Moreno Koch MC, Calvo C, Gonzalez S, Alvarez-Mon M. The immunosenescent phenotype in mice and humans can be defined by alterations in the natural immunity reversal by immunomodulation with oral AM3. Immunopharm Immunotoxicol 1997; 19: 53-74 [Medline].
19. Biron CA, Nguyen KB, Pien GC, Cousens LP, Salazar-Mather TP. Natural killer cells in antiviral defense: function and regulation by innate cytokines. Annu Rev Immunol 1999; 17: 189-220 [Medline].
20. Janeway CA, Travers P, Hunt S, Walport M. Host defense against infection. In: Immunobiology: the immune system in health and disease, 3rd ed. London: Current Biology Publications; 1997. p. 9.1-9.52.
21. Gallin JI. Disorders of phagocytic cells. In: Gallin JI, Goldstein IM, Snyderman R, editors. Inflammation: basic principles and clinical correlates, 2nd ed. New York: Raven Press; 1992. p. 859-874.
22. Wilson R. The role of infection in COPD. Chest 1998;113(Suppl):242S-248S.
23. Milvio C. Efficacy and safety of a new biological response modifier (AM3) in the prevention of recurrent acute infections in chronic obstructive bronchitis (COB) [Spanish]. Geriátrica 1990; 6: 308-312 .
24. Villarrubia VG, Calvo C, Romero M, Dominguez Cardona M, and Sada G. Therapeutic impact of AM3 (biological response modifier) on prevention of recurrent acute infections of the respiratory tract: analysis of 683 persons at high risk. Acta Toxicol Ther 1993;14:121-134.
25. Villarrubia VG, Domínguez Carmona M. Las infecciones agudas recidivantes en la EPOC en el medio laboral y prevención con Inmunoferón. Med Seguridad Trabajo 1997;45:1-20.
26.
Collet JP,
Shapiro P,
Ernst P,
Renzi T,
Ducruet T,
Robinson A.
Effects
of an immunostimulating agent on acute exacerbations and hospitalizations in patients with chronic obstructive pulmonary disease. The
PARI-IS Study Steering Committee and Research Group. Prevention
of Acute Respiratory Infection by an Immunostimulant.
Am J Respir
Crit Care Med
1997;
156:
1719-1724
27. Villarrubia VG, Sada G, Sozzani S, Luini W, Spreafico F. AM3 restores NK and macrophage antitumor cytotoxic activities in immunocompromised mice [Spanish]. Oncología 1987; 10: 283-291 .
28. Villarrubia VG, Herrerias JM, Alvarez-Mon M, Chirigos MA. Hepatitis B virus and the inflammatory/immunologic response (II): a new opportunity for the treatment of chronic hepatitis B and a suggestion for the treatment of other persistent viral diseases [Spanish]. Rev Esp Enferm Dig 1998; 90: 514-522 [Medline].
29. Moya P, Baixeras E, Barasoain I, Rojo JM, Ronda E, Alonso ML, Portoles A. Inmunoferón (AM3) enhances the activities of early-type interferon inducers and natural killer cells. Immunopharm Immunotoxicol 1987; 9: 243-256 [Medline].
30. Villarrubia VG, Valladolid JM, Elorza FL, Sada G, Vilchez JG, Jimenez M, Herrerias JM. Therapeutic response of chronic active hepatitis B (CAHB) to a new immunomodulator: AM3. Immunohematological effects. Immunopharm Immunotoxicol 1992; 14: 141-164 [Medline].
31. Sanchez L, Pena E, Civantos A, Sada G, Alvarez MM, Chirigos MA, Villarrubia VG. AM3, an adjuvant to hepatitis B revaccination in non-responder healthy persons. J Hepatol 1995; 22: 119-121 [Medline].
32. American Thoracic Society. Standards for the diagnosis and care of patients with chronic obstructive pulmonary disease. Am J Respir Crit Care Med 1995;152:S77-S120.
33.
Garcia-Suarez J,
Prieto A,
Reyes E,
Manzano L,
Merino JL,
Alvarez-Mon M.
Severe chronic autoimmune thrombocytopenic purpura is associated with an expansion of CD56+ CD3 natural killer cells subset.
Blood
1993;
82:
1538-1545
34. Prieto A, Reyes E, Garcia-Suarez J, Carrión F, Hernandez MP, Chafer J, Alvarez-Mon M. A low blood lymphocyte count is associated with an expansion of activated cytotoxic T lymphocytes in patients with B cell chronic lymphocytic leukemia. Eur J Haematol 1997; 59: 89-99 [Medline].
35. Hirt W, Nebe T, Birr C. Phagotest and Bursttest (Phagoburst), test kits for study of phagocyte functions [German]. Wien Klin Wochenschr 1994; 106: 250-252 [Medline].
36.
Takeuchi M,
Nagai S,
Izumi T.
Effect of smoking on natural killer cell
activity in the lung.
Chest
1988;
94:
688-693
37. Linden M, Larson M, Prellner T, Brattsand R, Laitinen LA. Seasonal variation in the function of blood monocytes obtained from healthy nonsmokers, asymptomatic smokers, and smokers with chronic bronchitis. Chronobiol Int 1994; 11: 266-272 [Medline].
38. Fietta A, Merlini C, De Bernardi PM, Gandola L, Piccioni PD, Grassi C. Non specific immunity in aged healthy subjects and in patients with chronic bronchitis. Aging (Milano) 1993; 5: 357-361 [Medline].
39.
Vogel L,
van Alphen L,
Geluk F,
Troelstra A,
Martin E,
Bredius R,
Eijk P,
Jansen H,
Dankert J.
Quantitative flow cytometric analysis of opsonophagocytosis and killing of nonencapsulated Haemophilus influenzae by human polymorphonuclear leukocytes.
Clin Diagnostic Lab
Immunol
1994;
1:
394-400
40. Murphy TF, Sethi S, Klingman KL, Brueggemann AB, Doern GV. Simultaneous respiratory tract colonization by multiple strains of nontypeable Haemophilus influenzae in chronic obstructive pulmonary disease: implications for antibiotic therapy. J Infect Dis 1999; 180: 404-409 [Medline].
This article has been cited by other articles:
 |
|
 |
|
  M. Miravitlles Review: Do we need new antibiotics for treating exacerbations of COPD? Therapeutic Advances in Respiratory Disease, October 1, 2007; 1(1): 61 - 76. [Abstract] [PDF]
|
|
|
|
 |
|
 N. Minematsu and S. D. Shapiro To Live and Die in the LA (Lung Airway): Mode of Neutrophil Death and Progression of Chronic Obstructive Pulmonary Disease Am. J. Respir. Cell Mol. Biol., August 1, 2007; 37(2): 129 - 130. [Full Text] [PDF]
|
|
|
|
 |
|
 D. Serrano-Gomez, R. T. Martinez-Nunez, E. Sierra-Filardi, N. Izquierdo, M. Colmenares, J. Pla, L. Rivas, J. Martinez-Picado, J. Jimenez-Barbero, J. L. Alonso-Lebrero, et al. AM3 Modulates Dendritic Cell Pathogen Recognition Capabilities by Targeting DC-SIGN Antimicrob. Agents Chemother., July 1, 2007; 51(7): 2313 - 2323. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 P. M. Henson, G. P. Cosgrove, and R. W. Vandivier State of the Art. Apoptosis and Cell Homeostasis in Chronic Obstructive Pulmonary Disease Proceedings of the ATS, August 1, 2006; 3(6): 512 - 516. [Full Text] [PDF]
|
|
|
|
 |
|
 K. Rydell-Tormanen, L. Uller, and J. S. Erjefalt Direct evidence of secondary necrosis of neutrophils during intense lung inflammation Eur. Respir. J., August 1, 2006; 28(2): 268 - 274. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 E. Reyes, A. Prieto, A. de la Hera, P. de Lucas, R. Alvarez-Sala, J. L. Alvarez-Sala, and M. Alvarez-Mon Treatment With AM3 Restores Defective T-Cell Function in COPD Patients Chest, March 1, 2006; 129(3): 527 - 535. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
M. Alvarez-Mon, M. Miravitlles, J. Morera, L. Callol, and J. L. Alvarez-Sala Treatment With the Immunomodulator AM3 Improves the Health-Related Quality of Life of Patients With COPD Chest, April 1, 2005; 127(4): 1212 - 1218. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 P. J. Barnes Mediators of Chronic Obstructive Pulmonary Disease Pharmacol. Rev., December 1, 2004; 56(4): 515 - 548. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 E. Gamble, D. C. Grootendorst, C. E. Brightling, S. Troy, Y. Qiu, J. Zhu, D. Parker, D. Matin, S. Majumdar, A. M. Vignola, et al. Antiinflammatory Effects of the Phosphodiesterase-4 Inhibitor Cilomilast (Ariflo) in Chronic Obstructive Pulmonary Disease Am. J. Respir. Crit. Care Med., October 15, 2003; 168(8): 976 - 982. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
P.J. Barnes, S.D. Shapiro, and R.A. Pauwels Chronic obstructive pulmonary disease: molecular and cellularmechanisms Eur. Respir. J., October 1, 2003; 22(4): 672 - 688. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
S. Inoue, H. Nakamura, K. Otake, H. Saito, K. Terashita, J. Sato, H. Takeda, and H. Tomoike Impaired Pulmonary Inflammatory Responses Are a Prominent Feature of Streptococcal Pneumonia in Mice with Experimental Emphysema Am. J. Respir. Crit. Care Med., March 1, 2003; 167(5): 764 - 770. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
M. Miravitlles Exacerbations of chronic obstructive pulmonary disease: when are bacteria important? Eur. Respir. J., July 1, 2002; 20(36_suppl): 9S - 19s. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
M. J. TOBIN Chronic Obstructive Pulmonary Disease, Pollution, Pulmonary Vascular Disease, Transplantation, Pleural Disease, and Lung Cancer in AJRCCM 2001 Am. J. Respir. Crit. Care Med., March 1, 2002; 165(5): 642 - 662. [Full Text] [PDF]
|
|
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
| Proc. Am. Thorac. Soc. | Am. J. Respir. Cell Mol. Biol. |