Controlled Clinical Laboratory Comparison of Two Supplemented Aerobic and Anaerobic Media Used in Automated Blood Culture Systems To Detect Bloodstream Infections

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Journal of Clinical Microbiology, March 1998, p. 657-661, Vol. 36, No. 3
0095-1137/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Controlled Clinical Laboratory Comparison of Two Supplemented Aerobic and Anaerobic Media Used in Automated Blood Culture Systems To Detect Bloodstream Infections

R. Ziegler,¹ I. Johnscher,¹ P. Martus,² D. Lenhardt,¹ and H.-M. Just¹^,^*

Institut für Klinikhygiene, Medizinische Mikrobiologie und Klinische Infektiologie, Klinikum Nürnberg, 90419 Nürnberg,¹ and Institut für Medizinische Statistik und Dokumentation, Universität Erlangen-Nürnberg, 91054 Erlangen,² Germany

Received 2 September 1997/Returned for modification 14 October 1997/Accepted 24 November 1997

	ABSTRACT

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A 20-ml blood sample was collected from adult patients with suspected bloodstream infections and distributed equally intothe four volume-controlled bottles of a blood culture set consistingof aerobic and anaerobic BACTEC Plus/F bottles and aerobic andanaerobic BacT/Alert FAN bottles. All bottles were incubated intheir respective instruments for a standard 5-day protocol oruntil the instruments signalled positivity. Samples in all bottleswith negative results by these instruments were terminally subcultured.A total of 8,390 blood culture sets were obtained during the studyperiod, of which 4,402 (52.5%) met the study criteria. Of these,946 (21.5%) were positive either by instrument signal or by additionalterminal subculture of all negative bottles and yielded growthof microorganisms. Five hundred eighty-nine (13.4%) blood culturesets were considered to have recovered 663 clinically significantorganisms. When both the BACTEC and the BacT/Alert systems wereused, 465 positive sets were detected; BACTEC alone detected 52positive sets and BacT/Alert alone detected 72 (P = 0.09). Nodifferences were found between the two systems in microbial recoveryrate from blood cultures obtained from patients on antibiotictherapy. Significantly more members of the family Enterobacteriaceae(P < 0.01) were detected from patients without antimicrobial therapyby BacT/Alert than by BACTEC. The false-negative rates were 0.20%for BACTEC and 0.32% for BacT/Alert. A significantly higher false-positiverate was found for BACTEC (P < 0.0001). Both systems were comparablefor the time to detection of microorganisms. However, gram-positivebacteria were detected faster by BACTEC and Enterobacteriaceaewere detected faster on average by BacT/Alert. We concluded thatboth systems are comparable in their abilities to recover aerobicand anaerobic organisms from blood cultures and a terminal subculturemight not be necessary for either of the two systems. The increasedpositivity rate when using an anaerobic bottle in a two-bottleblood culture set is due to the additional blood volume ratherthan to the use of an anaerobic medium.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Due to the high morbidity and mortality associated with bacteremia (7), the rapid detection and subsequent identificationof microorganisms from blood remain critical services of the clinicalmicrobiology laboratory. Numerous blood culture methods are available,and selecting the optimal system for the diagnostic laboratoryis an important and often difficult task (15). Many remarkableimprovements have been made in an attempt to reduce the time toisolate pathogens from blood. Advancements in the use of liquidmedia linked with automation technology have enhanced the abilityof laboratories to provide faster blood culture results. Two continuouslymonitored noninvasive blood culture systems, the BACTEC 9240 (BectonDickinson, Heidelberg, Germany) and the BacT/Alert (Organon Teknika,Eppelheim, Germany), are in widespread use. The main advantagesof the two systems over previous generations of blood cultureinstruments include full automation once the bottles are loaded,a shorter time to detection of blood pathogens, considerable laborsavings, and improved laboratory work flow. The BacT/Alert andthe BACTEC 9240 systems monitor the growth of organisms by checkingfor elaboration of CO₂ with a colorimetric and a fluorescent sensor,respectively.

New aerobic and anaerobic media were developed by the manufacturers to remove a variety of growth inhibitors from patients'blood, to enhance the recovery of fastidious organisms, and toimprove the detection of bacteremia and fungemia in patients receivingantimicrobial therapy. BACTEC Plus/F medium consists of soybean-caseindigest broth, primary supplements, and two types of resin, a nonionicabsorbing resin and a cation-exchange resin. FAN medium (BacT/Alert)is a brain heart infusion broth base containing Ecosorb, a proprietarysubstance that contains adsorbent charcoal, Fuller's earth, andother components.

A number of studies comparing the two systems have been carried out, but to our knowledge, none of them compared the supplementedaerobic and anaerobic BACTEC Plus/F media with the supplementedaerobic and anaerobic BacT/Alert FAN media in one controlled clinicaltrial.

This study was conducted to compare the performances of the two blood culture systems, BACTEC 9240 and BacT/Alert, in termsof microbial recovery, time to detection, and false-positive andfalse-negative rates, thereby indicating the performance of theaerobic and anaerobic BACTEC Plus/F resin media and the aerobicand anaerobic BacT/Alert FAN media.

	MATERIALS AND METHODS

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Patient population. This monocenter study was conducted from August 1995 through February 1997 in a 2,500-bed acute-care community hospital whichprovides a full range of medical and surgical care. The hospitalcares for an appreciable number of transplant, immunosuppressedpatients, as well as patients presenting common community-acquiredinfections. Blood cultures were obtained from all adult patientswith suspected bacteremia during the study period and processedin the hospital-related Institute of Microbiology and Hygiene.

Study design. Blood culture sets were prepared for the purposes of the study; each set contained four volume-controlled and randomized bottles,one each containing aerobic and anaerobic BACTEC Plus/F mediaand aerobic and anaerobic BacT/Alert FAN media. Written instructionsfor obtaining a blood culture, the required amount of blood, andthe order of inoculation of the bottles for clinicians were included.In respect of the patient and with the agreement of the ethicalcommission of our hospital, a 20-ml amount of blood for one bloodculture set was considered the maximum to obtain from a singlevenipuncture. This amount was distributed equally into each ofthe four bottles. The inoculum volume was determined in the microbiologylaboratory by weight. Sets in which any one of the bottles didnot contain a minimum of 3 ml of blood or in which the volumedifference between two bottles was more than 3 ml were considerednoncompliant and excluded from the study but processed for thebenefit of the patient.

On arrival in the laboratory, all bottles were placed in their respective instruments for a 5-day incubation time at 35°Cand monitored in accordance with the manufacturers' recommendations.FAN aerobic bottles were vented before incubation.

Bottles indicated as positive by the instrument as well as bottles positive on arrival were Gram stained. Based on the Gramstain result, aliquots of the bottles were subcultured onto adequatemedia (chocolate agar incubated at 35°C in a 5% CO₂-enriched atmosphereor blood agar with aerobic and anaerobic incubation at 35°C).All microorganisms were identified by standard microbiologic procedures.All false-positive bottles (i.e., bottles that were smear andsubculture negative after instrument signal) were replaced intothe instrument during the 5 days of protocol. A terminal blindsubculture onto chocolate agar and blood agar (aerobic and anaerobicincubation as described above) was performed for all negativebottles. False-negative bottles had no positive signal by theinstrument, but growth occurred on the terminal subculture.

Statistical methods. The following data of all blood cultures were entered in a computer database: collection time, loading time, blood volumeof each bottle, detection of growth by each bottle, growth onsubculture and identity of microorganisms recovered, antimicrobictherapy, and the detection time for each positive bottle. Detectiontime of a microorganism was defined as the time between loadinga blood culture bottle into the instrument and the time when apositive signal occurred followed by growth on subculture. Forcomparison of detection times, only clinically significant isolatesrecovered in both systems were taken into account. If both bottlesof one system recovered the same organisms, the shorter time todetection was taken into account for comparison. The clinicalimportance of isolated microorganisms was determined after consultationwith the patient's physician in accordance with published criteria(6, 10, 16, 18). Statistical analysis was done for bloodcultures meeting the study criteria. Only isolates classifiedas being clinically significant were taken into account. Sensitivitieswere calculated in two manners. For comparison of the two systems,the common denominator of positive cultures was determined byall four terminal blind subcultures. For evaluating the usefulnessof terminal subcultures in clinical routines, the detection rateof each system was determined with reference only to the relatedterminal subculture. The common denominator for the determinationof both the false-positive and the false-negative rates for eachsystem was the total of 4,402 compliant sets of the study. Themain scientific goal of the study was the comparison of the sensitivitiesand specificities of both systems. For these two analyses, theBonferroni correction was used. All other analysis on subgroupsof patients or isolates must be considered explorative withoutprotection against the error of multiple testing. All comparisonswere evaluated by McNemar's test ( $alpha$ = 0.05, two-sided) by usingthe statistical package SPSSWIN.

	RESULTS

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A total of 8,390 blood culture sets were obtained during the study period. Of these, 4,402 (52.5%) met the study criteria;of these, 946 (21.5%) yielded growth of 1,083 bacteria or fungi.Five hundred eighty-nine (13.4%) compliant sets, positive by eitherinstrument signal or terminal subculture only, detected 663 bacteriaor fungi that were considered clinically significant. Three hundredfifty-seven (8.1%) sets recovered only organisms classified ascontaminants.

Of the 589 positive blood culture sets with significant isolates, 508 (86.3%) were positive by BACTEC 9240 and 523 (88.8%)sets were positive by BacT/Alert. BACTEC alone detected 52 (8.8%)positive sets, and BacT/Alert alone detected 72 (12.2%). Withreference to the terminal blind subcultures of both systems, BACTECand BacT/Alert showed sensitivity rates of 86.3 and 88.8% respectively.With reference to the system-related terminal subculture, theBACTEC instrument demonstrated a detection rate of 98.3% and theBacT/Alert instrument gave one of 97.4%.

Nine false-negative blood cultures occurred with the BACTEC instrument (three Candida species and single isolates of Staphylococcusaureus, Streptococcus pneumoniae, Listeria monocytogenes, Enterobacteragglomerans, Pseudomonas aeruginosa, and Pseudomonas stutzeri)and 14 false negatives occurred with the BacT/Alert instrument(four P. aeruginosa, three Acinetobacter species, two Stenotrophomonasmaltophilia, two Candida species, and single isolates of Streptococcussanguis, Escherichia coli, and Proteus mirabilis).

The false-negative rates for the systems were 0.20% for BACTEC and 0.32% for BacT/Alert.

A significantly higher false-positive rate was found for BACTEC, 6.2%, than for BacT/Alert, 1.4% (P < 0.0001).

The comparative yields of bacteria and fungi from the two systems are indicated in Table 1. Of the 663 clinically significantorganisms from compliant sets, 482 (72.7%) were recovered fromboth systems, 80 (12%) were recovered by BACTEC only, and 101(15.2%) were recovered by BacT/Alert only. The differences observedin the recovery of bacteria reached statistical significance onlyfor the Enterobacteriaceae group. The BacT/Alert system detectedsignificantly more Enterobacteriaceae than the BACTEC system did(P < 0.01). A similar trend was seen in the recovery of yeastsfrom blood cultures obtained from patients without antibiotictherapy. For all other organisms, there were no significant differencesin the number of positive cultures between systems, neither byorganism group nor by species.

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TABLE 1. Comparative yields of clinically important bacteria and fungi in BACTEC Plus/F and FAN aerobic and anaerobic culture sets

Of all compliant blood culture sets, 41.9% (1,807 sets) were obtained from patients receiving antimicrobial therapy. Of the589 positive compliant sets with significant isolates, 35.5% (208)were obtained from patients receiving antibiotics. There wereno significant differences in isolation rates between the twosystems for patients receiving antibiotics. The BacT/Alert systemdetected significantly more Enterobacteriaceae than the BACTECsystem did (P < 0.01) from patients without antibiotic therapy.

The times to detection of several bacterial groups were compared for the two systems (Table 2). Gram-positive bacteria weredetected significantly faster by the BACTEC system, whereas Enterobacteriaceaeon average were recovered faster by the BacT/Alert system. Therewas no difference between the two systems in the cumulative percentageof positive cultures after 24, 48, and 72 h of incubation. Withinthe first 24 h, BACTEC detected 89.8% and BacT/Alert detected89.6% of the positive cultures; after 48 h, 95.7 and 96.9% weredetected by BACTEC and BacT/Alert, respectively; and after 72h, 99.0 and 99.4% were detected by the two systems, respectively.The average times to detection were 9.0 h for the BACTEC systemand 10.4 h for the BacT/Alert system (P < 0.05). The significantdifference in average time to detection between both systems wascaused by the higher detection rate within the first 6 h of theBACTEC instrument (50.7% detected by BACTEC and 45.8% by BacT/Alert).

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TABLE 2. Comparative speed of detection of clinically significant organisms when both systems were positive and detection time was provided for both systems (n = 421)

Delayed entry was defined as a time difference of >12 h between blood sample collection and placement of a blood culture bottleinto the respective instrument. More than half of the compliantpositive blood cultures had a transportation time of >12 h dueto the fact that our new hospital building is separated from thelaboratory. Delayed entry had no effect on the sensitivity ofthe BacT/Alert instrument, but for the BACTEC system, the detectionrate was significantly lower for blood cultures with delayed entrythan for those with no delay (P = 0.0097). Differences also occurredin detection of the Enterobacteriaceae group: BacT/Alert recoveredsignificantly more Enterobacteriaceae from blood cultures withdelayed entry than BACTEC did (P = 0.0062) when the subgroup ofpatients not receiving antibiotic therapy was considered.

The data of the two systems allow not only a system-versus-system comparison but also a comparison of the two media, i.e.,resin aerobic versus FAN aerobic media and resin anaerobic versusFAN anaerobic media (Table 3). No significant differences wereseen between the aerobic media nor between the anaerobic mediaof the two systems in terms of detection rate. A comparison ofthe aerobic and anaerobic media of each system showed significantdifferences. The false-positive rate was significantly higherfor both resin media than for the FAN media. The false-negativerates for both anaerobic media (4.7% for resin and 3.9% for FAN)were higher than those for the aerobic media (1.7% for resin and2.2% for FAN).

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TABLE 3. Detection of positive cultures and false-positive signals by aerobic and anaerobic media

Anaerobic bacteria causing septicemia were recovered from 13 compliant blood culture sets. Both systems detected four, theBACTEC system alone detected six, and the BacT/Alert system alonedetected three anaerobic bacteria.

	DISCUSSION

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This monocenter-controlled evaluation compared the performances of the supplemented aerobic and anaerobic BACTEC resin media,under identical conditions of observation against the supplementedaerobic and anaerobic BacT/Alert FAN media in a clinical trial.Simultaneous inoculation of all four bottles from a single bloodculture also enabled a system-versus-system comparison of theBACTEC 9240 and the BacT/Alert instruments. To our knowledge,no data have been published yet on this subject. In the past,several studies have evaluated the performance of the BACTEC (20)and BacT/Alert (2, 11) instruments, comparing either thetwo nonsupplemented media (19), the resin medium and the standardBacT/Alert medium (1, 9, 13), or the aerobic resin mediumand the aerobic FAN medium (4, 8, 14). Outcomes have beenquite different: the BACTEC system detected significantly moregram-positive cocci and the BacT/Alert system recovered significantlymore Enterobacteriaceae in a first comparison (19) of the twononsupplemented media.

Auckenthaler et al. (1) as well as Smith et al. (13) compared BACTEC resin medium to standard BacT/Alert medium, andboth groups reported a better performance in terms of microbialrecovery, false-positive rate, and detection time for the resinmedium. A comparison of aerobic resin medium with aerobic FANmedium in a recent multicenter (4) study has demonstrated equalresults. The previous single-center study by Pohlman et al. (8)showed a better recovery rate for Enterobacteriaceae and Pseudomonasby use of the BacT/Alert system with fewer false-positive results.In comparison with the results of other studies (4, 11, 12,17), the positivity rate of blood cultures in our study washigh (21.5% positive sets), with 13.4% sets recovering clinicallysignificant organisms. With the exception of members of the Enterobacteriaceaegroup, which were recovered significantly (P < 0.01) more oftenby the BacT/Alert system alone, there were no significant differencesin terms of microbial recovery between the two systems. The Enterobacteriaceaethat were detected significantly more frequently by the BacT/Alertsystem resulted from blood cultures from patients without antimicrobialtherapy. There was also a tendency towards a similar result forthe fungi group: BacT/Alert detected slightly more Candida sp.isolates from patients without antibiotics than from patientswith antimicrobial therapy. However, these are results of an explorativeanalysis in which, due to the small numbers of cases, a high betaerror and the problems of multiple testing must be taken intoaccount.

Reports of high false-negative rates, up to 6% (12, 13), suggest that terminal subculturing of negative BACTEC culturesafter 5 days of incubation may be necessary, whereas others havesuggested that this is not needed in the BacT/Alert system (3).In our trial, the false-negative rates were similarly low forboth systems (0.20% for BACTEC and 0.32% for BacT/Alert) and thesensitivities for the BACTEC and BacT/Alert instruments with referenceto the related terminal subcultures were 98.3 and 97.4%, respectively;therefore, we have concluded that a blind terminal subculturemay not be necessary for either of the two systems.

The introduction of automated blood culture systems also serves the purpose of reducing the routine workload for laboratorypersonnel. A low false-positive rate is one important factor here.Our results showed a significantly (P < 0.0001) higher false-positiverate for the aerobic and anaerobic resin media (6.2%) than forthe FAN media (1.4%). During the study period, both instrumentswere used in accordance with the recommendations and specificationsof each manufacturer. Laboratory facilities were equal for bothsystems. All false-positive blood cultures were replaced intothe instrument, incubated for the rest of the 5-day incubationperiod, and terminally subcultured. A small percentage of thefalse-positive signals by the BACTEC instrument occurred afteran electricity breakdown, which did not affect the BacT/Alertinstrument.

Due to the need to reduce laboratory costs, many microbiology laboratories do not have 24-h coverage by technical personnel.Especially in smaller hospitals, there is no microbiology laboratoryavailable, so that blood cultures must be sent to external laboratories.Therefore, a delay may occur from the time blood is drawn untilthe bottle is placed into a blood culture instrument. Our hospitalconsists of an original building complex with 1,500 beds and anew building with 1,000 beds which is situated 10 km away. Allblood specimens from the new building must be transferred to thelaboratory in the original building, so that a delay of >12 hmay occur.

Those blood cultures that were obtained after the microbiology laboratory was closed for the day were collected in a centrallaboratory that is open 24 h per day and were incubated at 35°C,so that almost all blood cultures with delayed entry were preincubatedat 35°C. Delayed entry did affect the sensitivity of the BACTECinstrument in that the detection rate was significantly lowerfor blood cultures with delayed entry than for those with no delay(P = 0.0097).

The numbers of false-negative sets with delayed entry and of false negative sets with a transport time of <12 h were too smallfor valid comparison. For the BACTEC system, 6 of 9 false-negativesets were sets with delayed entry; for BacT/Alert, 8 of 14 falsenegatives were sets with delayed entry. In spite of the smallnumber, there seems to be no need for blind terminal subcultureeither for sets with overnight preincubation at 35°C or for setsprocessed within the first 12 h after collection. Both systemsdetected organisms faster from culture sets with delayed entrysince these sets were preincubated. With regards to the handlingof preincubated blood culture bottles, the BacT/Alert system offersthe advantage of a visible change on the bottom of a positivebottle so that the bottle can be processed onto subcultures beforeincubation into the instrument. The interpretation of Gram stainresults for positive bottles was more difficult for FAN mediathan for resin media due to the charcoal particles in the media.

Staphylococcus epidermidis, which is considered a contaminant, was recovered more frequently from the FAN aerobic bottle (n= 424) than from the resin aerobic bottle (n = 349); this morefrequent recovery may be due to the fact that the FAN aerobicbottle must be vented before incubation in the instrument. Theuse of needles to manually vent the aerobic FAN bottles may increasethe probability of contaminating the bottle.

The question whether there is any advantage to using both aerobic and anaerobic blood culture media routinely (5) or whetheranaerobic media should be used for the detection of bacteremiaonly in patients at risk of having an anaerobic infection is oftenraised. Only 13 positive blood cultures out of 589 sets with clinicallysignificant organisms recovered anaerobic bacteria, 11 being isolatedfrom the anaerobic medium only and 2 being isolated from boththe aerobic and anaerobic media. Four of the 11 blood culturesets with obligate anaerobic bacteria represented polymicrobialsepticemia; in addition to the anaerobic bacteria, Enterobacteriaceae,Staphylococcus aureus, and Candida spp. were isolated from thecorresponding aerobic bottle as well. Definitively, seven (1.2%)blood cultures with monomicrobic obligate anaerobic pathogenswould not have been detected by using only an aerobic bottle.By using the anaerobic resin bottle in addition to the aerobicone, the detection rate increased by 10.2%, with facultative anaerobicbacteria contributing 8.7% and obligate anaerobic bacteria contributing1.6%. Analogously, the anaerobic FAN bottle increased the positivityby 9%, of which 8% was due to facultative anaerobic bacteria and1% was due to strict anaerobic ones. Diagnoses of patients withsepticemia due to obligate anaerobic bacteria included colitisulcerosa, pancreatitis, diabetes mellitus with erysipelas, cholangitis,leukemia, and pneumonia, so that anaerobic infections could havebeen expected. According to Weinstein et al. (17), an increasein the volume of blood inoculated into BacT/Alert aerobic bottles(from 5 to 10 ml) increased the overall yield (7.2%) of clinicallyimportant organisms. From our results and those reported by Weinsteinet al. (15, 17), we conclude that the higher recovery rateachieved when the anaerobic bottle is included is due to the inoculationof a larger blood volume rather than to the use of an additionalanaerobic medium.

In summary, both systems are comparable for recovering clinically significant microorganisms from adult patients with bacteremiaand fungemia receiving antibiotic therapy at the time of bloodculture collection. With blood from patients without antibiotictherapy, the BacT/Alert system detected significantly more Enterobacteriaceae.The high false-positive rate of the BACTEC system caused additionalwork and material costs in our laboratory. With the BacT/Alertinstrument, the software capabilities were more convenient forthe user, and failure rarely occurred.

	ACKNOWLEDGMENTS

This study was supported in part by grants from Becton Dickinson and Organon Teknika.

	FOOTNOTES

^* Corresponding author. Mailing address: Institut für Klinikhygiene, Medizinische Mikrobiologie und Klinische Infektiologie,Klinikum Nürnberg, Flurstr. 17, 90419 Nürnberg, Germany. Phone:(49) 911 398 2522. Fax: (49) 911 398 3266.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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