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15 March 1996 | Volume 124 Issue 6 | Pages 539-547
Background: Nasal carriage of Staphylococcus aureus is common among health care workers, but outbreaks caused by such carriers are relatively uncommon. We previously reported outbreaks of S. aureus skin infections that affected newborn infants and were attributed to an S. aureus nasal carrier who had had an associated upper respiratory tract infection (URI) during the outbreak period.
Objective: To investigate the contribution of a nasal methicillin-resistant S. aureus (MRSA) carrier (physician 4) who contracted a URI to an outbreak of MRSA infections that involved 8 of 43 patients in a surgical intensive care unit during a 3-week period.
Design: An epidemiologic study of an outbreak of MRSA infections and a quantitative investigation of airborne dispersal of S. aureus associated with an experimentally induced rhinoviral infection.
Setting: A university hospital.
Participants: 43 patients in a surgical intensive care unit and 1 physician.
Measurements: Molecular typing was done, and risk factors for MRSA colonization were analyzed. Agar settle plates and volumetric air cultures were used to evaluate the airborne dispersal of S. aureus by physician 4 before and after a rhinoviral infection and with or without a surgical mask.
Results: A search for nasal carriers of MRSA identified a single physician (physician 4); molecular typing showed that the MRSA strain from physician 4 and those from the patients were identical. Multivariate logistic regression analysis identified exposure to physician 4 and duration of ventilation as independent risk factors for colonization with MRSA (P < equals 0.008). Air cultures showed that physician 4 dispersed little S. aureus in the absence of a URI. After experimental induction of a rhinovirus URI, physician 4's airborne dispersal of S. aureus without a surgical mask increased 40-fold; dispersal was significantly reduced when physician 4 wore a mask (P < equals 0.015).
Conclusions: Physician 4 became a "cloud adult," analogous to the "cloud babies" described by Eichenwald and coworkers who shed S. aureus into the air in association with viral URIs. Airborne dispersal of S. aureus in association with a URI may be an important mechanism of transmission of S. aureus.
The nose (anterior nares) is the most common body site of colonization on health care workers; frequencies range between 20% and 90% [12, 20-22]. Although many factors have been shown to increase S. aureus nasal colonization [23-29], nasal carriage alone does not cause outbreaks. If it did, the high frequency of nasal carriage of S. aureus by hospital personnel would be associated with a similarly high frequency of outbreaks. This is not the case, which suggests that other factors must modify the state of the nasal carrier of S. aureus for an outbreak to occur.
The likelihood that a nasal carrier of S. aureus will cause an outbreak may increase if the carrier acquires the ability to disperse the organism into the air. Airborne dispersal of S. aureus is uncommon and directly related to the quantity of S. aureus colonizing the anterior nares [30]. No more than 10% of healthy nasal carriers of S. aureus disperse the organism into the air [17, 31], and males disperse more commonly than females [32]. A viral upper respiratory tract infection (URI) was shown to change newborn infant nasal carriers of S. aureus from nondispersing to dispersing status, creating so-called "cloud babies" who can cause outbreaks [33]. Similar studies have not been done in adults. We previously reported a nasal carrier of S. aureus who was linked to outbreaks in two newborn nurseries in association with URI, and we postulated the existence of a "cloud adult" [2].
In the present study, we identified a nasal carrier of methicillin-resistant S. aureus (MRSA) as the probable cause of an outbreak of nosocomial MRSA infections in a surgical intensive care unit. During the outbreak period, this carrier had developed a URI. It was subsequently shown that this carrier could not disperse S. aureus into the air in the absence of a URI, but after infection with a rhinovirus, he began to disperse S. aureus into the air around him, thus becoming a "cloud adult."
Outbreak Investigation
In early April 1994, the infection control department at our institution became aware of several cases of MRSA pneumonia in a surgical intensive care unit. A microbiology database query showed that, during a 3-week period in late March and early April 1994, 8 of 43 patients in the surgical intensive care unit had acquired MRSA. This was a clear increase from baseline (Figure 1). ARTICLE
A Cloud Adult: The Staphylococcus aureus-Virus Interaction Revisited
Nosocomial outbreaks of Staphylococcus aureus infection have been well described. They occur most commonly in special care units, such as newborn nurseries [1-9], neonatal intensive care units [10-12], surgical intensive care units [13, 14], and burn units [15], and they have also been reported in patient wards [16, 17] and operating rooms [18, 19]. Factors associated with nosocomial outbreaks of S. aureus include the overuse of antibiotic agents, inadequate handwashing, understaffing, and health care workers carrying the organism [1-19].
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Our study had two major components. First, we investigated the epidemiology of an outbreak of MRSA infections, and our results suggested that a nasal carrier of MRSA who had an associated URI played a causative role. Second, we investigated the effect of an experimentally induced rhinovirus URI on this same nasal carrier's ability to disperse MRSA into the air.
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The charts of all eight patients colonized with MRSA were reviewed using the Centers for Disease Control criteria for nosocomial infection [34]. The temporal relations among the patients developing colonization or infection with MRSA are shown in Figure 2. Seven of the eight patients were from the same surgery service; all seven were intubated and had sputum samples growing MRSA; and five of these seven met criteria for MRSA nosocomial pneumonia. The eighth patient had leukemia, was on an internal medicine service, and developed nosocomial MRSA bacteremia (patient 6). The tight clustering of the first five cases and the fact that all surgical patients were colonized first in their respiratory tracts suggested a common mechanism of transmission.
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Sixty-four of 70 (91%) clinical personnel (33 nurses, 13 physicians, and 18 respiratory therapists) who had worked in the surgical intensive care unit during the outbreak period were cultured for nasal carriage of MRSA. A sterile swab moistened with phosphate-buffered saline (pH, 7.2) was used to culture both anterior nares, was plated on tryptic soy agar (BBL, Cockeysville, Maryland) containing 4 µg of oxacillin per mL, and was incubated at 37 °C for 48 hours. The identity of S. aureus was confirmed by using the slide coagulase test (Staphyloslide Test, Becton Dickinson, Cockeysville, Maryland). Resistance to methicillin was verified by using both an agar diffusion method [35] and a microtiter tube dilution method [36] at 35 °C; all isolates were resistant to methicillin and to several other antibiotic agents. Only physician 4, a resident in training, tested positive for MRSA.
Physician 4 was interviewed immediately after his S. aureus isolate was confirmed to be MRSA. He described having had a persistent URI during the period in which the patients were colonized (1 March 1994 to 22 March 1994; Figure 2). The URI had lasted 3 weeks and had been characterized by extensive nasal discharge, coughing, and occasional sneezing. Physician 4 had received azithromycin during the last week of his illness. He reported washing his hands after sneezes and before sterile procedures; during this period, he wore a mask only during operating room procedures. Because he had already switched to a nonclinical elective at the time he was interviewed, removal from patient care activities was unnecessary. He received nasal treatment with mupirocin four times per day for 1 week in late June. Although the nasal culture done immediately after mupirocin treatment was negative for S. aureus, a culture done 18 days later was positive for methicillin-sensitive S. aureus (MSSA). No further infection control measures were taken, because no increase in MSSA infections had been detected. During 3 months of follow-up surveillance, no additional patients with MRSA infection or colonization in the surgical intensive care unit were identified (Figure 1).
We reviewed the charts of all 43 patients who were present in the surgical intensive care unit during the period in which physician 4 had the URI to determine whether contact with physician 4 or any other physician was an independent risk factor for MRSA colonization. Physician contacts were determined by counting the number of times that the physician operated on, examined, or did a procedure on a patient (counts were based on the presence of the physician's signature or name in the patient's chart). Additional data collected from the charts included age, sex, duration of hospitalization before admission to the surgical intensive care unit, duration of stay in the surgical intensive care unit before the URI period, duration of stay in the intensive care unit during the URI period, number of invasive procedures, Glasgow coma score at the time of admission to the surgical intensive care unit, number of different antibiotics used during the URI period, number of days receiving each antibiotic during the URI period, number of contacts with each physician during the URI period, wound debridement, intubation, abdominal surgery, thoracic surgery, abdominal trauma, chest trauma, previous hospitalizations, previous nursing home residences, MSSA colonization or infection, and death.
Effect of Rhinoviral Infection on Airborne Dispersal of Staphylococcus aureus
After we obtained approval from our institutional review board, physician 4 gave informed consent to participate in a study to determine the effect of an experimental rhinovirus URI on physician 4's ability to disperse S. aureus into the air. All air cultures were done in a small conference room (20 ft x 16 ft x 8 ft [2560 ft3]; 6 air changes/h). Air cultures were done before the physician entered the room (baseline) and then with the physician in the room both before and after rhinoviral infection and with and without a surgical mask (Anago, Fort Worth, Texas). In the period before the rhinoviral infection, air cultures were done at 10 a.m. (with no mask) or 2 p.m. (with mask), or both, after the room had been occupied for other purposes.
Because of scheduling difficulties with physician 4, air cultures in the period after the viral infection were done at 8 a.m. (with mask) and 9 a.m. (with no mask) when the room had been unoccupied since 5 p.m. the previous day. The mask was worn first to minimize carryover of S. aureus in the air from the 8 a.m. period to the 9 a.m. period. Nose and skin surface cultures were done to determine whether the viral infection changed the number of S. aureus present at different body sites.
Air cultures were done using two methods—settle plates and a volumetric air sampler—as shown in Figure 3. Forty-one agar plates (Columbia agar with 5% sheep blood, Carr-Scarborough Microbiologicals, Stone Mountain, Georgia) were placed on top of a conference table (8 ft x 8 ft) in the middle of the room for 1 hour to culture S. aureus that settled out of the air. In addition, a two-stage volumetric air sampler (Graseby Andersen, Atlanta, Georgia) containing two blood agar plates was used for three 20-minute periods to culture organisms that might have been too small to fall onto the settle plates (Figure 3). The air sampler cultures 1 ft3/minute. All agar plates were incubated for 48 hours at 37 °C, and all colonies with morphology consistent with S. aureus were tested for coagulase activity and methicillin susceptibility, as described above. All isolates identified as S. aureus were saved for subsequent typing.
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Quantitative Mucosal and Skin Surface Cultures
Cultures of physician 4 at two mucosal sites (anterior nares and posterior pharynx) and selected skin sites (midline anterior chest, midline abdomen, axilla, and groin) were done using sterile cotton swabs moistened with phosphate-buffered saline. For skin cultures, a sterile template (5 cm x 5 cm) was placed on the skin, and a moistened cotton swab was rubbed twice over the area. Each swab was placed in 5 mL of sterile tryptic soy broth (BBL), sonicated for 1 minute, vortexed for 15 seconds, and then serially diluted and surface plated (0.1 mL) on blood agar. Colonies with typical S. aureus morphology were further evaluated as described above.
Rhinoviral Infection
Physician 4 was screened for contraindications to rhinoviral infection [37]. The rhinovirus used was a strain of type 39 that had been safety tested [38] and used in volunteer studies at the University of Virginia [39, 40]. A serum sample drawn from physician 4 before infection had a neutralizing antibody titer to rhinovirus type 39 of less than 1:2. The virus inoculum contained 100 tissue culture infectious doses50 in a 1 mL volume [41] and was administered through intranasal drops (0.25 mL per nostril) on two occasions 10 minutes apart using a sterile 1-mL pipette.
The illness was defined by a modification [37] of the scoring method of Jackson and coworkers [41]. Symptoms were evaluated daily for 5 days by using a nine-item questionnaire. A clinical cold was defined as a total symptom score greater than 6 and either the subjective impression of having developed a cold or 3 or more days of self-reported rhinorrhea. Nasal washings were collected 2 days before and 3 and 19 days after viral inoculation for viral culture in human embryonic lung cells (WI38). Physician 4 refused more frequent nasal wash collections. Serum specimens taken before and 6 weeks after viral inoculation were tested for homotypic neutralizing antibody.
Staphylococcus aureus Typing by Analysis of Chromosomal DNA
Isolates of S. aureus were stored in 20% milk at –70 °C after verification that each organism was S. aureus. Typing was done by using a modification of the method of Goering and Duensing [42, 43]. Chromosomal DNA was isolated by plating S. aureus on tryptic soy agar and incubating overnight at 37 °C. Cells were centrifuged at 1900 g for 15 minutes, the cell pellet was suspended in 1 mL of 0.85% NaCl, and 20 µL was transferred to a tube containing 400 µL of EC buffer (6 mmol/L tromethamine, 1 mol/L NaCl, 100 mmol/L ethylenediaminetetraacetic acid [EDTA], 0.5% Brij 58, 0.2% deoxycholate, 0.5% sarkosyl at pH 7.5). In rapid succession, 20 µL of lysostaphin (20 mg/mL; Applied Microbiology, New York, New York) and 450 µL of 2% InCert agarose (FMC, Rockland, Maine) were added with agitation. The mixture was poured into a plug mold, cut into 1-mm thick slices, and incubated in EC buffer at 37 °C for 4 hours. The slices were washed with Tris-EDTA buffer (100 mmol/L of tromethamine and 100 mmol/L of EDTA) for three 20-minute periods, then 1 mL of EDTA-sarkosyl buffer (0.4 mol/L EDTA [pH 9.3] and 1% sarkosyl) and 50 µL of proteinase K (20 mg/mL; Promega, Madison, Wisconsin) were added, and the slices were incubated overnight at 50 °C. The slices were washed with Tris-EDTA buffer for three 20-minute periods and stored at 4 °C.
For restriction endonuclease digestion, slices were washed in buffer as suggested by the manufacturer (25 mmol/L tromethamine-acetate [pH 7.8], 50 mmol/L of potassium acetate, and 10 mmol/L of magnesium acetate; Promega) for three 20-minute periods. A 4 mm x 4 mm x 1 mm piece was then cut, placed in a 96-well microtiter plate containing 50 µL of digestion buffer that contained 12 units of Sma I (Promega), and incubated at 25 °C for 8 hours. The plugs were incorporated into a 1% agarose gel (SeaKem LE, FMC). Electrophoresis was done using a CHEF DR-II apparatus (BioRad, Hercules, California) using 0.5 times tris-borate-EDTA buffer at 13 °C, a pulse ramp of 5 to 50 seconds, and a run time of 23 hours. A 
ladder pulsed field gel electrophoresis marker (New England Biolabs, Beverly, Massachusetts) was used as a molecular weight standard. Gels were stained with ethidium bromide (0.5 µg/mL) and photographed using ultraviolet light. Banding patterns were compared by visual inspection. For organisms with the same antibiotic susceptibilities, different strains were defined as having more than three band differences.
Data Analysis
Data from the 8 patients colonized with MRSA were compared with data from the 35 noncolonized patients in several ways. Univariate analysis was done by using the Fisher exact test, the chi-square test (Epistat Services, Richardson, Texas), the Student t-test, or the Mann-Whitney rank-sum test (Minitab, State College, Pennsylvania). Because of the small number of total patients, it was not possible to use all of the variables in a multivariate logistic regression model (Statistical Analysis System, SAS Institute, Cary, North Carolina) at one time. Therefore, only variables that were statistically significant by univariate analysis plus age, sex, and Glasgow coma scale at the time of admission to the surgical intensive care unit were analyzed further using a forward stepwise approach.
The air culture data were analyzed by using a general linear model (SAS Institute) controlling for day, use of a mask, distance of plate from physician 4, and plate location. Only days when data were collected both with and without a mask were analyzed: days 1 and 3 (before viral infection) and 6 through 10 (after viral infection). We conservatively adjusted P values using the Dunn-Sidack method, a slight variation on the Bonferroni method.
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The results of univariate analysis of MRSA risk factors are shown in Table 1. Factors that were significantly different (P < 0.05) between MRSA-colonized and noncolonized patient groups included duration of stay in the surgical intensive care unit during the URI period, number of invasive procedures during the URI period, number of different antibiotic agents used during the URI period, number of days receiving antibiotic agents during the URI period, number of intubation days during the URI period, and number of physician contacts. Physicians 1, 2, 3, and 4 had the most contacts with the patients in the surgical intensive care unit, and they were all significantly associated (P < 0.05) with case-patients. They were all surgical residents and were all said by their supervising attending physicians to have good aseptic technique. A total of 15 physicians had contact with patients in the surgical intensive care unit during the URI period; none of the other 11 physicians had significantly greater contacts with the MRSA-colonized patient group than did physicians 1, 2, 3, and 4 (P > 0.05).
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Forward stepwise regression analysis was then used to determine which of the factors associated with MRSA colonization by univariate analysis were independent risk factors for MRSA colonization. When all 43 patients were considered, only two variables were found to be independently associated with MRSA colonization: duration of ventilation (P = 0.007) and contact with physician 4 (P = 0.008). When data from the 42 surgical patients (excluding the patient on the medical service) were analyzed in the same way, physician 4 was still independently associated with MRSA colonization (P = 0.002).
Rhinovirus Cold of Physician 4
Nasal cultures taken from physician 4 three days after viral inoculation grew rhinovirus type 39. Cultures taken 2 days before and 19 days after viral inoculation were negative for virus. Physician 4 also had a greater than fourfold increase in serum neutralizing antibody (from less than 1:2 to 1:16) to rhinovirus type 39. He met the criteria for a common cold 3 and 4 days after viral inoculation (Figure 4); his illness consisted of sneezing, a runny nose, nasal stuffiness, a mild sore throat, and occasional coughing. His symptom score on the last day that air cultures were done was only 2. Notably, during the time that air cultures were done, physician 4 did not cough or sneeze.
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Mucosal and Skin Cultures of Physician 4
The results of physician 4's nasal cultures for S. aureus during the period of experimental rhinoviral infection are shown in Table 2. From the anterior nares, MSSA was isolated every time, but MRSA was isolated only once. In contrast, during the outbreak investigation, when agar containing oxacillin was used for cultures, MRSA was found each of the two times the nose was cultured, suggesting that the presence of MSSA obscured the detection of MRSA during the rhinovirus experiment. The throat and skin sites were cultured on 5 different days (1, 3, 6, 8, and 10 June). No MRSA isolates were detected, and MSSA was found on only three occasions (on 3 June in the abdomen and on 10 June in the left axilla and in the abdomen). The three MSSA skin isolates were typed, and all were identical to the MSSA strain found in the nose.
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Airborne Dispersal of Staphylococcus aureus from Physician 4
The air around physician 4 was cultured 17 different times for periods of 1 hour. From 797 plates, a total of 6554 colony-forming units (CFUs) of bacteria were isolated. Of these, 69 isolates (1.5%) were S. aureus. Organisms other than S. aureus were not defined at the species level. The pattern of isolation of all bacterial species (Figure 4, top) showed several interesting points. During the baseline period before the rhinoviral infection, approximately twice as many organisms were isolated in one culture interval (day 2) than in the other two sampling periods. On that day (Figure 4, top), physician 4 talked on the telephone most of the hour; he did not talk at all during any other culture periods. After viral infection, the number of CFUs isolated showed a clear upward trend whether physician 4 was (correlation coefficient, r = 0.81) or was not (r = 0.98) wearing a mask. No evidence suggested that wearing a mask decreased the total number of CFUs in the air.
The volumetric air sample plates grew 5 to 10 times as many bacteria as the settle plates in a 1-hour period. The volumetric air cultures had 2 to 3 times as many organisms on the smaller particle size plates (< 5 microns, bottom plate) as were found on the larger particle size plates (> 5 microns, top plate). When physician 4 was in the room, a clear gradient of organisms was in the air; that is, the number of organisms decreased as the distance from physician 4 increased. The mean numbers of CFUs detected by the top plate were 16.7 ± 10.0 CFUs (mean ±SD) at 2 feet from physician 4 and 8.3 ± 4.7 CFUs at 4 feet (P = 0.009, Student t-test). For the bottom plate, the mean numbers of CFUs were 32.0 ± 13.7 CFUs at 2 feet compared with 21.9 ± 11.1 CFUs at 4 feet (P = 0.04, Student t-test).
All 69 S. aureus isolates from physician 4 were tested for susceptibility to oxacillin; 4 isolates (5.8%) were resistant (all from day 9; Figure 4, bottom). Twenty-seven of these organisms were studied using molecular typing, and representative strains are shown in Figure 5. In the period before viral infection, all 8 S. aureus organisms isolated were typed. Only 2 of 8 isolates came from physician 4. The baseline cultures were done immediately after periods in which persons worked in the conference room. The S. aureus from the baseline period that were not from physician 4 probably came from personnel working in the conference room just before the culture periods. Only the two S. aureus strains that came from physician 4 were used for further analysis (Figure 4, bottom).
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Sixty-one S. aureus organisms were grown in the period after the viral infection. Nineteen isolates were chosen for typing (see Figure 4, bottom): all 8 isolates from days 6 through 8, 3 of 10 isolates from day 9 without mask, 4 of 43 isolates from day 10 without mask, and 4 of 10 isolates from day 10 with mask. The strains of all 19 S. aureus isolates were shown to be the same as those isolated from physician 4. In our subsequent analysis and in producing Figure 4, we assumed that the 42 remaining S. aureus isolates also came from physician 4. The lack of "background noise" (S. aureus not attributable to physician 4) in the period after viral infection was attributed to the fact that no one had been in the conference room for at least 12 hours.
The S. aureus data from days 1, 3, and 6 through 10 were further analyzed using a general linear model. The dependent variable was the number of S. aureus CFUs attributable to physician 4 that was detected on each agar plate. When physician 4 did not wear a mask, the number of S. aureus CFUs per plate was significantly greater when physician 4 was infected with rhinovirus on day 10 than when he was not infected on days 1 and 3 (0.83 ± 0.14 CFUs compared with 0.0 ± 0.0 CFUs; adjusted P < equals 0.015). On day 10 during the rhinoviral infection period, the mean number of S. aureus CFUs per plate was significantly less when physician 4 wore the mask than when he did not (0.14 ± 0.06 CFUs compared with 0.83 ± 0.14 CFUs; adjusted P < equals 0.015). Not surprisingly (Figure 4, top), the effect of the mask was significantly different on different days (P < equals 0.0001).
On day 10 when physician 4 was not wearing a mask, the distribution of the S. aureus isolates from air cultures was remarkable. Twenty-nine of the 47 agar plates (61.7%), including all settle plates at the extremes of distance from physician 4, grew S. aureus. The 6 volumetric culture plates grew 9 S. aureus isolates, and 23 settle plates grew 34 S. aureus isolates. Nineteen days after viral inoculation, physician 4 had no S. aureus detectable by air culture.
Relatedness of Staphylococcus aureus isolates from Physician 4 and Patients
Physician 4 had two strains of S. aureus in his nose: one MSSA strain and one MRSA strain. His nasal carriage of these two organisms was stable during a 3-month period (Figure 5). Strains of MRSA were available from 6 of 8 patients, and all 6 had the same type as the MRSA strain found in physician 4's nose.
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Given that physician 4 had nasal colonization with MSSA and MRSA simultaneously, it is interesting that no outbreak of MSSA infections occurred. This was probably related to the fact that almost all patients in the surgical intensive care unit during the MRSA outbreak period received parenteral antibiotics, either prophylactically or therapeutically, that were active against MSSA but not MRSA. The azithromycin received by physician 4 while he had a URI may also have suppressed the MSSA, but not the MRSA, in his nose.
The most interesting feature of this outbreak was that physician 4 acquired a URI during the time he was thought to have transmitted S. aureus to patients. Subsequent efforts in our investigation focused on whether the URI may have increased the likelihood of transmission. Most existing evidence suggests that S. aureus is transmitted in the hospital setting through direct contact with the hands of personnel [22]. We previously speculated [2] that airborne transmission of S. aureus from a nasal carrier might occur in association with a URI. This same consideration was raised by Nahmias and coworkers [44] in their investigation of an outbreak of S. aureus surgical site infections attributed to a single surgeon and by Boyce and colleagues [17] in connection with an MRSA outbreak associated with a respiratory therapist who had chronic MRSA sinusitis. The best evidence supporting this mechanism was provided by Eichenwald and coworkers [33], who showed that a viral URI caused babies who carried nasal S. aureus to disperse the organism into the air and become "cloud babies" with the ability to cause outbreaks.
Our baseline air cultures showed that few S. aureus organisms were shed into the air around physician 4 under resting conditions. Hare and Thomas [45] found that when agar plates were held directly under the nose of resting nasal S. aureus carriers for 5 minutes, no organisms were detectable. Using a more sensitive volumetric air sampler method to culture the air inside a closed chamber containing a volunteer, Bethune and coworkers [32] found that few nasal carriers of S. aureus dispersed organisms into the air, even when exercising. Notably, extensive talking by physician 4 did not affect S. aureus dispersal, although it essentially doubled the total number of organisms other than S. aureus that were isolated from the air (Figure 4).
After rhinoviral infection, the total number of bacteria in the air around physician 4 increased steadily, but little effect on S. aureus was seen until the second day of physician 4's symptomatic cold, when the number of dispersed S. aureus CFUs increased. One day later, when cold symptoms had started to wane, the number of S. aureus CFUs in the air increased even more. These S. aureus organisms were widely dispersed around physician 4; 62% of all agar plates were growing the organism, and all plates at maximum distances to the front, side, and back of physician 4 were growing the organisms. Thus, in association with a rhinovirus URI, physician 4 was surrounded by S. aureus in the air and became a "cloud adult" analogous to the "cloud babies" described by Eichenwald and coworkers [33]. The mechanism for this effect is unclear at this time, although it may be as simple as the URI swelling the nasal turbinates, resulting in very narrow air passages. This, in turn, would lead to high-speed, turbulent air flow over a wet surface, which could create an aerosol.
Although it is unfortunate that physician 4 was not cultured longer so that the duration of the "cloud adult" effect could be clearly defined, lack of this later culture data does not detract from our goal, which was to determine whether "cloud adults" existed. We have confirmed this possibility, and it is now important to investigate the incidence of "cloud adults," the duration of the phenomenon in those who manifest it, whether the phenomenon occurs with all or just certain URIs, and which preventive interventions need to be considered for health care workers or patients with URIs. Until more data are available, our findings should not be extrapolated to other health care workers.
If further studies show that the "cloud adult" phenomenon is generalizable to most nasal S. aureus carriers, then the potential implications of these findings would be far reaching. Twenty percent to 90% of health care workers who care for patients are nasally colonized with S. aureus [12, 19-22]. Because adults average two colds per year [46], "cloud adults" may be working around patients all year long. If this is so, then interventions to minimize the spread of S. aureus to patients are necessary. Our results suggest one possible intervention. The statistically significant reduction in the number of S. aureus CFUs found when physician 4 wore a mask, in combination with the fact that none of the patients on whom physician 4 operated during the outbreak period developed surgical site infections, suggest that surgical masks may interrupt the airborne transmission of S. aureus from the nose. This phenomenon could also be relevant to the transmission of other bacterial pathogens that colonize the nose [47], such as Streptococcus pneumoniae, Streptococcus pyogenes, Haemophilus influenzae, and Neisseria meningitidis [48, 49].
Drs. Reagan and Thomas: Primary Care (IIA), Mountain Home Veterans Affairs Medical Center, PO Box 4000, Mountain Home, TN 37684.
Mr. Hampton, Ms. Robertson, and Mr. Streed: Medical Center Boulevard, North Carolina Baptist Hospitals, Inc., Winston-Salem, NC 27157.
Ms. Hoen: Department of Public Health Sciences, PPII, Bowman Gray School of Medicine, 2000 West 1st Street, Winston-Salem, NC 27157.
Dr. Gwaltney: Department of Internal Medicine, University of Virginia Health Science Center, Charlottesville, VA 22908.
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References
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