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Neonates suffering from group B streptococcal (GBS) pneumonia often lack type-specific opsonizing
antibodies. We studied the influence of combined intratracheal treatment with surfactant and a specific antibacterial polyclonal antibody (IgG fraction) on bacterial proliferation and lung function in an
animal model of GBS pneumonia. Near-term newborn rabbits received an intratracheal injection of
either the specific IgG antibody, nonspecific IgG, surfactant, a mixture of surfactant and the antibody, or 0.9% saline. At 30 min the rabbits were infected with a standard dose (108) of the encapsulated GBS strain 090 Ia. After 5 h of mechanical ventilation the mean estimated increase in bacterial
number in lung homogenate (log10 colonies/g) was 0.76 in the antibody group, 0.92 in the nonspecific IgG group, 0.55 in the surfactant group, and 1.29 in the saline group. A mean decrease in bacterial number (
0.05) was observed in the group that received combined treatment with surfactant
and antibody (p < 0.05 versus all other groups). Lung-thorax compliance was significantly higher in
both groups of surfactant-treated animals compared with saline or IgG treatment. We conclude that
in experimental neonatal GBS pneumonia combined treatment with surfactant and a specific immunoglobulin against GBS reduced bacterial proliferation more effectively than either treatment alone.
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INTRODUCTION |
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ABSTRACT
INTRODUCTION
METHODS
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Group B streptococci (GBS) are a common cause of systemic infections in the neonatal period. One to four per thousand newborn infants suffer from early-onset GBS septicemia and although nowadays only few term newborn infants die from the disease, mortality is disturbingly high in infected premature babies (1). Most premature infants with systemic or pulmonary GBS infections have respiratory symptoms (1, 2), and data from animal experiments and limited clinical experience seem to indicate that in these patients respiratory failure is in part caused by surfactant deficiency. We have previously identified a GBS strain pathogenic to rabbits and developed an animal model to study the effect of surfactant in ventilated newborn rabbits after intratracheal infection with GBS (3). In preterm newborn rabbit fetuses with experimentally induced GBS pneumonia, surfactant replacement therapy improved lung function and mitigated intrapulmonary bacterial proliferation (4). There is also evidence from mostly uncontrolled clinical trials that surfactant treatment can improve gas exchange in babies with congenital GBS pneumonia (5).
Infants of mothers who lack type-specific antibodies to the GBS polysaccharide capsule are especially prone to severe infections (8). Thus active and passive immunization against GBS has been proposed (9, 10). The present study was designed to test the hypothesis that combined intratracheal treatment with surfactant and a specific antibacterial immunoglobulin (IgG) could improve lung function and mitigate bacterial proliferation in experimental neonatal GBS pneumonia.
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INTRODUCTION
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Bacteria
An abundantly encapsulated low-density (LD) phase variant of GBS
(gift from Stellan Håkansson, University of Umeå, Umeå, Sweden) was
processed from the reference strain 090 Ia Colindale by repeated gradient centrifugation. It was stored in aliquots at 70° C, precultured,
washed, centrifuged, and suspended in normal saline at a concentration of approximately 109 live bacteria per milliliter as determined by
spectrophotometric measurement of the optical density at 595 nm.
Additionally, the actual number of colony-forming units (cfu) in the
suspension was determined for each individual experiment by colony
counting (3).
Antibody
A polyclonal antibody to GBS 090 Ia LD was generated in adult
rabbits by repeated intravenous injection of heat-killed bacteria as
previously described (11). The IgG fraction was purified by affinity
chromatography (Protein A, Sephadex 6 MB; Kabi Pharmacia, Stockholm, Sweden) and ultrafiltration (Amicon Centriplus 100; Amicon,
Witten, Germany). The final product contained > 99% IgG as judged
by cellulose/acetate foil serum electrophoresis (LMB, Bad Godesberg, Germany). The capacity of this antibody to stimulate the release
of reactive oxygen metabolites during phagocytosis of GBS by polymorphonuclear neutrophils (PMN) was tested using the nitroblue tetrazolium (NBT) test (12). The antibody was dissolved in normal saline
at a concentration of 5 mg/ml and stored in aliquots at 70° C until use.
Surfactant
Curosurf (Chiesi Farmaceutici, Parma, Italy) is a modified natural surfactant isolated from minced pig lungs that has been characterized (13) and tested in various clinical trials before. Curosurf and the specific antibody were mixed in proportion 1:1 and incubated for 30 min at 37° C before use. The final concentrations of surfactant and IgG in the suspension given to the animals were 40 mg/ml and 2.5 mg/ml, respectively.
In Vitro Experiments
Influence of IgG on surface tension. The influence of rabbit IgG
(Sigma Chemicals, St. Louis, MO) on the surface activity of Curosurf,
suspended in normal saline at a concentration of 2 mg/ml or 5 mg/ml,
was tested in a Pulsating Bubble Surfactometer (Electronetics Corporation, Buffalo, NY). IgG was added at concentrations ranging from 1 to 40 mg/ml and the sample was incubated at 37° C for 30 min before
analysis. Measurements were made at 37° C during 50% cyclic area
compression at a rate of 40 min
1. Surface tension at minimum bubble
size (
min) was recorded after 5 min of pulsation.
Influence of surfactant and antibody on release of reactive oxygen metabolites by polymorphonuclear leukocytes. Phagocytes can kill bacteria by release of reactive oxygen metabolites. PMN were isolated and purified from healthy adult donors as described previously (12). Both the encapsulated (GBS LD) and the nonencapsulated phase variant (GBS HD) of the GBS strain were used for these studies. The bacteria (3 × 108) were heat-killed and incubated with 5 × 105 PMN, specific IgG antibody (8.5 mg/ml), and/or surfactant (4 mg/ml) on ELISA plates (12). Commercially available nonspecific rabbit IgG and normal saline were used as controls. Oxygen metabolite release was measured spectrophotometrically by means of the NBT reduction test (12).
Animal Experiments
Animals. Eleven pregnant New Zealand White rabbits were obtained from local suppliers. Rabbit fetuses were delivered by cesarean section (3 to 11 animals per litter) at a gestational age of 29.5 d as previously described (3). Term gestation for rabbits is 30 to 31 d. Previous studies on lung function demonstrated that dynamic compliance at 29.5 d is not significantly different from that of term animals (14). During the operation the doe was anesthetized and supplemental oxygen was delivered via a face mask.
Experimental protocol. The rabbit fetuses were anesthetized, paralyzed, and tracheotomized at birth and allocated in a random order to five different treatment groups. Using a specially designed tracheotomy tube with an indwelling wedged plastic catheter tubing (inner diameter, 0.75 mm; Portex, Hythe, Kent, UK), 5 ml/kg body weight (bw) of the antibody preparation (corresponding to 12.5 mg/kg bw of IgG) with or without surfactant (200 mg/kg bw) were instilled immediately into the liquid-filled lungs before the onset of ventilation. Controls received the same volume of the nonspecific rabbit IgG preparation, surfactant, or normal sterile saline. At 30 min all experimental groups received an intratracheal bolus injection of 5 ml/kg of the GBS suspension. Before reconnecting the animals to the ventilator system, the instilled liquid was moved from the central airways to peripheral airspaces by injecting three times 10 ml/kg bw of air with a microsyringe. The exact number of cfu given to each individual rabbit was calculated from the injected volume and the determination of cfu/ml in the infectious inoculum. The five treatment groups that originated from this procedure will be referred to in the following as: (1) specific IgG, (2) nonspecific IgG, (3) saline, (4) surfactant, and (5) surfactant + specific IgG.
All animals were then transferred to a warmed multiplethysmograph system (14) and ventilated in parallel in sealed Plexiglas chambers with a common ventilator as previously described (3, 4, 14). Peak
inspiratory pressure was individually adjusted for each animal to obtain a tidal volume of 6 to 10 ml/kg bw. Stabilization of tidal volumes
was obtained within 15 min after birth. Lung-thorax compliance (ml × kg1 × cm H2O1) was calculated from the quotient of tidal volume
and peak inspiratory pressure. The animals were ventilated for 5 h.
Recordings were obtained at 0, 15, 30, 45, 60, 90, 120, 150, 180, 210, 240, 270, and 300 min. Electrocardiogram (ECG) was recorded at the
same intervals and animals were counted as survivors if the heart rate was > 100 beats per min without evidence of arrhythmia or atrioventricular block. At the end of the experiments the rabbits were killed
and the chest was opened. Blood from the right cardiac ventricle was aspirated for blood culture (Bactec Plus blood culture system; Becton
Dickinson, Sparks, MD). A heparinized sample was taken for blood
gas analysis.
The left main bronchus was tied and the left lung was excised, divided in two parts of approximately equal size by a frontal section, and weighed. The peripheral part was placed immediately into the sterilized tube of a tissue homogenizer (Kontes Scientific Glassware Instruments, Vineland, NJ) and stored on ice until further processing.
Bronchoalveolar lavage. The right lung remained in situ and was
lavaged via the tracheal cannula. 0.9% saline with heparin (2 U/ml) at
room temperature was instilled into the lungs via the tracheal cannula
at a volume of 20 ml/kg bw. This volume was washed in and out three
times, and the procedure was repeated four times with an average recovery of 83 ± 9%. The lavage fluid from each animal was pooled and
centrifuged at 150 × g for 10 min. The resulting pellet was collected
and saline was added to obtain a final volume of 1 ml of cell suspension. One hundred microliters of this suspension was stained with Giemsa-Romanowski stain and the cells were counted in a Bürker chamber and a flow cytometer. Cytospin preparations from the rest of the
suspension were stained with May-Grünwald-Giemsa stain and used
for differential counting of inflammatory cells. The supernatant was
stored at 70° C and its protein content was analyzed (protein assay;
Bio-Rad Laboratories, Munich, Germany).
Bacterial counting. The weight of the lung specimens was adjusted to 1 g with sterile normal saline. The samples were homogenized with a high-speed (15,000 rpm) nylon microchamber tissue homogenizer (Sorval Omnimix; Dupont Instruments, Newton, CT). A serial dilution was performed and the diluted suspensions were spread on blood agar plates for colony counting after 24 h incubation. As bacterial proliferation follows a logarithmic growth curve, the results were expressed as mean log10 cfu/g lung (wet weight). The calculated number of cfu given to the rabbit (cfu/rabbit) represents a good estimate of the number of cfu in the lung of the rabbit (cfu/g lung) at the beginning of the experiments, as the bacteria were administered intratracheally and the total lung weight of a term rabbit is approximately 1 g (3). In a previous study we observed a very close correlation between the number of GBS instilled into the airways and the number of live bacteria detected in the left lung of animals killed 1 min after the injection (3). A positive difference between cfu/g lung after 5 h of ventilation and cfu/rabbit at the beginning of the experiment thus indicates bacterial growth, a negative difference indicates a decrease in the number of viable bacteria in lung homogenate.
Histologic examination. The central part of the left lung was fixed in 4% formalin and subsequently embedded in paraffin. Longitudinal sections were cut in a standardized fashion. The slides were coded, so that the investigator was unaware of the experimental condition of the animals. The specimens were examined by light microscopy with special reference to intra-alveolar edema, hyaline membranes, and airway epithelial necrosis. The influx of inflammatory cells was estimated using a semiquantitative grading system as previously described (3). Severe pneumonia was defined as an inflammatory reaction involving more than 30% of total lung parenchyma.
The study design and the management of the animals complied with national legislation. The trial protocol was approved by the local ethics committee for animal research.
Statistical Analysis
Data are given as mean ± SD or median and range. Values for lung
weight and physiological data were subjected to analysis of variance
(ANOVA) using the CRISP software program (Crunch Software, San
Francisco, CA). Between-group differences were evaluated by Student-Newman-Keuls' test. Differences in the incidence of complications between the groups were analyzed with the 
2 test. The limit
level of statistical significance was defined as p = 0.05.
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RESULTS |
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In Vitro Experiments
Surface tension measurements. Addition of IgG at concentrations 
1 mg/ml did not influence the low minimum surface
tension (min) of Curosurf diluted to 2 mg/ml (Figure 1). Only
at concentrations 
2 mg/ml did IgG cause an elevation of
min, indicating surfactant inactivation. When Curosurf was
tested at a concentration of 5 mg/ml, an IgG concentration
of 40 mg/ml was necessary to inhibit surface activity. These
data indicate that the presence of IgG in surfactant at a weight
ratio of 1:20 as used for our animal experiments probably does
not interfere with the surface properties of Curosurf.
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Oxygen metabolite release by PMN. The nonencapsulated (HD) variant of GBS 090 Ia strongly stimulated the release of reactive oxygen species from PMN (Figure 2). The encapsulated strain (GBS LD) had no such effect in itself; only after incubation with the specific IgG antibody was stimulation observed. The increased NBT reduction was not suppressed by adding surfactant to the incubation medium (Figure 2).
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Animal Experiments
Characterization of the experimental groups. Of 79 delivered fetuses, seven demonstrated ECG abnormalities already at the beginning of the experiments and were therefore excluded from further evaluation. Twenty-five other animals with normal initial ECG developed bradycardia < 100 beats/min or ECG abnormalities before the end of the 5-h experimental period and were also excluded from the final data analysis. No significant differences in survival rate (range, 56 to 67%) were found between the groups. Pneumothorax was found in one animal. Mean birth weight, final heart rate, tidal volume, and PCO2 of the remaining 47 rabbits are shown in Table 1. Final PCO2 in heart blood was significantly lower in both groups receiving surfactant, reflecting improved ventilation.
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Bacterial proliferation. A similar dose of bacteria was given
to all groups (Figure 3). Over the study period there was
prominent bacterial proliferation (all figures are log10 cfu differences between values representing the beginning and the
end of the experiment) in both the saline (+1.29) and the nonspecific IgG controls (+0.92). Slightly less bacterial growth
was observed in the animals receiving the specific anti-GBS-IgG (+0.76, not significant). Significantly less bacteria (p <
0.01) were detected in the lungs of infected rabbits treated
with surfactant than in those receiving saline at the same timepoint (Figure 3), but bacterial proliferation also occurred in
this group (+0.55). In contrast, animals receiving the mixture
of surfactant and the specific IgG showed no increase in bacterial number over the 5-h study period (0.05, p < 0.05 versus
all other groups). Blood cultures were positive for GBS in all
animals except four receiving the combined treatment with surfactant and specific IgG (Table 1).
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Lung-thorax compliance. At 15 min no significant differences in dynamic lung-thorax compliance were found between the groups. Compliance increased between 15 and 30 min in most animals, probably reflecting resorption of fetal lung liquid. Animals treated with saline or specific or nonspecific IgG showed a subsequent gradual decrease in dynamic compliance over the observation period. Animals receiving surfactant had significantly higher compliance values and maintained improved lung function throughout the experiments. Rabbits treated with specific IgG together with surfactant had similar compliance values as those receiving only surfactant. At 300 min compliance in each of the two surfactant-treated groups was significantly higher than in the three other groups (Figure 4).
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Bronchoalveolar lavage fluid (BALF). No significant differences in the total number of inflammatory cells were noted between the groups (Table 2). PMN were the predominant cell type in the majority of animals. About 10% of the inflammatory cells were represented by alveolar macrophages with only few lymphocytes being present. Total protein content was similar in lavage fluid in all groups (Table 2).
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Histological findings. All animals except five showed evidence of pneumonia with accumulation of inflammatory cells (mostly PMN) in alveoli and peripheral conducting airways (Table 2). In 29 rabbits the inflammatory reaction was classified as severe, i.e., involving more than 30% of the lung parenchyma, but there were no differences in the degree of inflammation between the groups. In 17 of the 47 rabbits there was prominent airway epithelial necrosis, again without differences between the groups. Hyaline membranes, absent or discrete in all but one of the 19 surfactant-treated rabbits, were prominent in 17 of 28 rabbits in the three groups that did not receive surfactant (p < 0.05).
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DISCUSSION |
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Encapsulated GBS need opsonization by specific antibodies in order to be phagocytized by polymorphonuclear neutrophilic granulocytes (PMN). Systemic disease in neonates has been associated with lack of these specific antibodies that are normally transferred in utero from the mother (8). Animal studies using monoclonal antibodies have demonstrated the benefit of specific, parenterally applied antibodies in the treatment of GBS infections (15). Clinical studies are far more difficult to evaluate as the commercially available IgG preparations often lack sufficient levels of type-specific opsonizing antibodies (16). Prevention strategies such as selective chemoprophylaxis or active immunization of pregnant women are currently being evaluated (9, 10). Our in vitro experiments confirm that nonencapsulated GBS are effectively taken up by PMN even in the absence of specific antibodies, whereas an encapsulated but otherwise identical strain needs opsonization by specific IgG. Surfactant does not interfere with the release of oxygen metabolites from PMN, stimulated by GBS in the presence of specific IgG.
On the other hand, immunoglobulins, like other proteins, may inhibit surfactant function. However, the inhibitory capacity of immunoglobulins is far below that of fibrinogen or albumin (17). The hyperimmune serum prepared for the present study can be used in extremely low concentrations and did not influence dynamic surface tension in our pulsating bubble measurements at IgG:surfactant weight ratios much larger than those used in our animal experiments. This is in keeping with our observation that admixture of IgG to surfactant did not inhibit its therapeutic effect on compliance in GBS-infected newborn rabbits. Also it is reassuring that data from a recent small clinical study, evaluating the use of aerosolized IgG in infants with respiratory syncytial virus (RSV) infections, did not demonstrate serious side effects on lung function (18). The possibility to administer specific antibodies as an aerosol with or without surfactant could have obvious clinical implications, as it might allow treatment of spontaneously breathing patients at an early stage of pulmonary infection, not yet requiring endotracheal intubation.
GBS often invade the neonatal lung via colonized amniotic fluid. Intra-alveolar accumulation of leaking plasma proteins, bacterial degradation products, and substances released from neutrophils (e.g., oxygen radicals, proteases including elastase) can result in a secondary surfactant dysfunction comparable to the acute respiratory distress syndrome (ARDS) in older patients (19). Data from clinical pilot studies suggest that surfactant can be used successfully in newborns with congenital pneumonia (5) but that the response to surfactant treatment is slower than in babies with uncomplicated respiratory distress syndrome. Although initial data from animal experiments published by Sherman and coworkers (20) indicated impaired macrophage function after surfactant treatment, more recent data from the same group demonstrated no stimulatory effects of commercially available modified natural surfactant preparations on the proliferation of GBS neither in vitro nor in newborn rabbits (21). In previous experiments using the same animal model we have shown that surfactant treatment actually mitigates streptococcal growth (3, 4). The mechanisms behind this effect are not clearly understood. Besides a direct bacteriostatic effect of surfactant, prevention of atelectasis and reduced accumulation of proteins in the alveoli might be important factors. Keeping the airways open throughout the respiratory cycle is probably crucial for effective mucociliary clearance. In the present study, histological examination of the lungs revealed no differences in the degree of cellular inflammatory reaction between the groups, although hyaline membranes were less prominent in animals receiving surfactant. For technical reasons (cutting of the left lung) no perfusion fixation under standardized distending pressures was performed. We therefore made no attempts to evaluate the alveolar expansion pattern in various treatment groups. Noninfected animals receiving the same volume of saline were not studied in the present series, but we know from previous experience that such control animals do not show any significant recruitment of granulocytes to the airspaces during a 5-h period of mechanical ventilation (3).
Besides its well-characterized biophysical properties, surfactant is probably of major importance in both the antibacterial and the antiviral defense system of the lung (22) and beneficial effects of exogenous surfactant on lung function have been reported in animal models of bacterial (4, 23), protozoal (24), or viral (25, 26) pneumonia. To some extent, these effects have been linked to the hydrophilic surfactant proteins SP-A and SP-D, which are both important stimulants of macrophage function. An increased susceptibility to GBS was recently described in genetically SP-A-deficient mice exposed to a relatively low dose of bacteria (27). However, these animals did not develop severe pneumonia and continued spontaneous breathing. In contrast, blocking of endogenous SP-A with a monoclonal antibody did not enhance bacterial proliferation in an experimental model of GBS pneumonia, similar to that employed in the present study (28). Further work is therefore required to define the precise role of the hydrophilic surfactant proteins (SP-A and SP-D) in the antibacterial defense system of the neonatal lung.
Intravenous administration of antibiotics is standard treatment for neonates with respiratory distress until bacterial infection can be ruled out by means of negative cultures. However, with conventional treatment drug levels might be low in the alveolar spaces and bacterial resistance against antibiotics is a widespread clinical problem, especially in adults. Bacteria opsonized by specific IgG antibodies are phagocytized and consequently killed intracellularly. This is a potential advantage as bacterial toxins or cell wall components of extracellularly killed microorganisms can cause severe adverse systemic reactions such as endotoxin shock or pulmonary hypertension. In patients affected by severe pneumonia, topical immunoglobulins might therefore serve as an adjunct to standard antimicrobial therapy.
It seems likely that simultaneous instillation of surfactant facilitates spreading of drugs in the peripheral airspaces, as previously shown for radiolabeled sulfur colloids administered via the airways together with surfactant (29). Other investigators documented the effectiveness of surfactant as a vehicle for a variety of pharmacological substances including antibiotics (30), lysozyme (31), antioxidants (32), and corticosteroids (33). A recent study describing the use of surfactant as a carrier for an adenovirus vector (34) introduces the possible use of surfactant in gene therapy.
We conclude that combined treatment with surfactant and a specific antibacterial antibody improves lung function and mitigates bacterial growth in experimental GBS pneumonia in ventilated newborn rabbits. The possible role of surfactant as a "vehicle" for various drugs administered via the airways deserves further evaluation.
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Footnotes |
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Correspondence and requests for reprints should be addressed to Egbert Herting, M.D., Department of Pediatrics, University of Göttingen, Robert-Koch Str. 40, D-37075 Göttingen, Germany. E-mail: eherting{at}med.uni-goettingen.de
(Received in original form October 14, 1998 and in revised form January 19, 1999).
Acknowledgments: The authors acknowledge the skillful work and technical assistance of Bim Linderholm, Eva Lundberg, Petru Popa, and Gabriele Walter. Surfactant for the studies was generously supplied by Serono Germany (Munich, Germany) and Serono Nordic (Solna, Sweden).
Supported by the Deutsche Forschungsgemeinschaft (DFG He 2072/2-2), the Swedish Medical Research Council (Project No. 3351), Konung Oscar II:s Jubileumsfond, and a collaborative project of the German Academic Exchange Service and the Swedish Institute.
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References |
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ABSTRACT
INTRODUCTION
METHODS
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DISCUSSION
REFERENCES
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27. LeVine, A. M., M. D. Bruno, K. M. Huelsman, G. F. Ross, J. A. Whitsett, and T. R. Korfhagen. 1997. Surfactant protein A-deficient mice are susceptible to group B streptococcal infection. J. Immunol. 158: 4336-4340 [Abstract].
28. Herting, E., D. S. Strayer, C. Jarstrand, B. Sun, and B. Robertson. 1998. Lung function and bacterial proliferation in experimental neonatal pneumonia in ventilated rabbits exposed to monoclonal antibody to surfactant protein A. Lung 176: 123-131 [Medline].
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