Detection of Bacteriocins by Matrix-Assisted Laser Desorption/Ionization Time-of-Flight Mass Spectrometry

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Applied and Environmental Microbiology, May 1999, p. 2238-2242, Vol. 65, No. 5
0099-2240/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Detection of Bacteriocins by Matrix-Assisted Laser Desorption/Ionization Time-of-Flight Mass Spectrometry

Natisha L. Rose, Peter Sporns, and Lynn M. McMullen^*

Department of Agricultural, Food and Nutritional Science, University of Alberta, Edmonton, Alberta T6G 2P5, Canada

Received 18 September 1998/Accepted 8 February 1999

	ABSTRACT

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The use of matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF MS) for the detection ofbacteriocins was investigated. A 30-s water wash of the sampleon the MALDI-TOF MS probe was effective in removing contaminantsof the analyte. This method was used for rapid detection of nisin,pediocin, brochocin A and B, and enterocin A and B from culturesupernatants and for detection of enterocin B throughout itspurification.

	TEXT

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Bacteriocin-producing lactic acid bacteria and purified bacteriocins have the potential for use as biopreservatives to extendstorage life or to enhance the safety of foods. Bacteriocins areproteinaceous compounds produced by lactic acid bacteria thatexhibit activity against closely related bacteria, and they mayalso be active against species beyond the same ecological niche(17).

Currently, researchers rely on bioassays such as deferred inhibition and agar diffusion tests for the detection of bacteriocinproduction and the determination of bacteriocins in foods (20).Such methods are indirect because they rely on a sensitive indicatororganism that varies among laboratories. In addition, the resultsare expressed in arbitrary units (AU), which vary with experimentalconditions (i.e., pH, temperature, nutrients, and choice of indicator)(6, 13).

A sensitive, rapid detection method for bacteriocins could be a useful method to track purification procedures, to detectbacteriocin production in experiments involving genetic manipulation,and to detect bacteriocins in foods (6, 20). Detecting thebacteriocin by searching for a compound with the appropriate molecularmass is one method of confirming the presence of bacteriocinsin cultures or food products. Matrix-assisted laser desorption/ionizationtime-of-flight mass spectrometry (MALDI-TOF MS) appears to havepotential as one suchmethod.

MALDI-TOF MS was first recognized in 1988 as a method of examining large molecules (16). With rapid advances in this technology,MALDI-TOF MS is becoming an essential tool in the analysis ofbiopolymers, including peptides and proteins. Generally, MALDI-TOFMS involves ion formation using a pulsed UV laser beam to depositenergy into a cocrystallized matrix-analyte sample and ejectionof the sample into a vacuum for desorption analysis. The majoradvantages of MALDI-TOF MS over other mass spectrometric techniquesare (i) its ease of use, (ii) its picomole-to-femtomole sensitivity(22), (iii) its high-mass (>200,000-Da) range and ability togive molecular mass values with a reported accuracy of ±0.1% orbetter (4, 5, 7, 22), and (iv) its relative toleranceto contaminants in the sample (5, 24, 25, 27). Theseadvantages make MALDI-TOF MS technology suitable for the analysisand characterization ofbacteriocins.

MALDI MS is usually used in conjunction with TOF mass analyzers that give a defined time of ion generation and are compatiblewith the pulsed lasers of MALDI MS (7). The TOF of the ionthrough the drift region is proportional to the mass/charge (m/z)ratio of the ion, which allows for the determination of mass.MALDI-TOF MS systems have also greatly advanced with the implementationof delayed extraction (3, 7, 14, 23, 25). Delayedextraction has been reported to significantly improve the resolvingpower, detection sensitivity, signal-to-noise (S/N) ratios, andmass measurement accuracy of MALDI-TOF MS (7, 14, 23, 25,27).

Presently, MALDI-TOF MS is recognized as a valuable tool for molecular mass measurements and is showing promise as a quantitationtool. MALDI-TOF MS has been used routinely for the analysis ofsynthetic peptides and proteins. However, the analysis of peptidesand proteins extracted from biological sources has been hamperedby the presence of contaminants, such as salts, glycerol, anddetergents (1, 4, 5, 18, 26, 27). These contaminantsmay suppress the peptide and protein signals completely. Sodiumdodecyl sulfate and salts have been shown to interfere with thesignal obtained for bovine serum albumin and cytochrome c (1,24). Wang et al. (24) reported that differences in salt contentamong samples might result in detection of certain peptides andproteins over others, yielding different mass spectral patternsand consequently poor spectrumreproducibility.

In bacteriocin purification, the presence of detergents such as Tween in All-Purpose Tween (APT) and de Man, Rogosa and Sharp(MRS) medium, both commonly used for the growth of bacteriocin-producingorganisms, may interfere with the analysis. Tween 80 is an essentialmedium component for bacteriocin production and detection (12,15). It is likely that partial purification of bacteriocin preparationswill be necessary to obtain a clean sample for analysis by MALDI-TOFMS; however, purification methods are often time-consuming, resultin the loss of biological material, and may even introduce morecontaminants that are incompatible with MALDI-TOF MS (26).

Researchers have investigated the use of activated synthetic membranes as an alternative to stainless steel in MALDI-TOF MSanalysis. By spotting a sample onto a membrane such as polyethylene,contaminants can be washed away, leaving the peptides and proteinsintact at the surface for analysis (4, 5, 26). This processresults in equal or greater sensitivity and mass resolution forall samples compared to those desorbed from stainless steel. Syntheticmembranes are particularly suitable for high-mass (i.e., >30,000-Da)molecules because severe ion suppression is typically observedin the analysis of high-mass mixtures (4, 5). Other researchershave used or suggested further processing of the sample on theprobe, such as a wash with cold water to remove the contaminants(18, 24, 27).

In this study, we developed a MALDI-TOF MS method for the detection of bacteriocins in culture supernatant and used the methodto determine the fate of a bacteriocin throughout a purificationprocedure.

Bacterial strains and media. The bacteriocin-producing lactic acid bacteria used in this study are listed in Table 1. Enterococcus faecium CTC 492 wasobtained from M. Hugas (Institut de Recera i Technologia Agroalimentàries,Girona, Spain), and E. faecium BFE 900 was isolated from blackolives by Franz et al. (8). Carnobacterium divergens LV13,obtained from B. G. Shaw (Institute of Food Research, Langford,Bristol, United Kingdom), and Lactobacillus sake ATCC 20017 wereused as sensitive indicator organisms against the producer strains.Frozen stock cultures were maintained at $-$ 70°C in Bacto APT broth(Difco Laboratories, Detroit, Mich.) supplemented with 20% glycerol(vol/vol). Prior to experimental use, Lactococcus lactis ATCC11454, Brochothrix campestris ATCC 43754, Pediococcus acidilacticiPAC-1.0, E. faecium CTC 492 and BFE 900, and C. divergens LV13cultures were subcultured twice and grown overnight in APT broth.L. sake ATCC 20017 was subcultured twice and grown overnight inlactobacillus MRS broth (Difco) prior to use. Solid agar mediumwas prepared by adding 1.5% (wt/vol) granulated agar (Difco) toeither APT or MRS media. Soft APT and MRS agar were prepared with0.75% agar (wt/vol).

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TABLE 1. Bacteriocin-producing organisms used in this study and characteristics of their bacteriocins

Preparation of culture supernatant. L. lactis ATCC 11454, P. acidilactici PAC-1.0, B. campestris ATCC 43754, and E. faecium CTC 492 and BFE 900 were grown for18 h at 30°C in 10 ml of APT broth. One-milliliter aliquots ofeach grown culture were pipetted into Eppendorf tubes and boiledfor 1 min. Cells were removed by centrifugation at 10,000 × gfor 10 min at 4°C. The supernatant fluid was collected and storedat 4°C until used for analysis, within 1day.

Purification of enterocin B. Enterocin B was purified by the method described by Franz et al. (9). E. faecium BFE 900 was grown for 18 h in 1 literof APT broth supplemented with 3% glucose (vol/vol). The culturewas heated for 30 min at 75°C, and cells were removed by centrifugation(8,000 × g; 30 min). The supernatant was collected and loadedonto an Amberlite XAD-8 column (150 by 75 mm; BDH Chemical Ltd.,Poole, United Kingdom). The column was washed with 1 liter of0.1% trifluoroacetic acid (TFA) and then with 750 ml of 30% ethanolin 0.1% TFA. The active fraction, as determined by a spot-on-lawnassay, was eluted with 60% ethanol in 0.1% TFA and concentratedto approximately 75 ml by a rotary evaporation. The concentratedfraction was adjusted to pH 4.5 with 20 mM sodium acetate buffer(SAB; pH 5). The fraction was loaded onto an SP Sepharose FastFlow cation exchange column (110 by 13 mm; Pharmacia Biotech,Baie D'Urfe, Quebec, Canada), and the column was sequentiallywashed with 100 ml of SAB, 60 ml of 100 mM sodium chloride inSAB, and 60 ml of 500 mM sodium chloride in SAB, which elutedthe bacteriocin. This active fraction was loaded onto a Sep PakC₁₈ reverse-phase column (Waters Ltd., Mississauga, Ontario, Canada).The column was washed with 10 ml of milli-Q water and then with10 ml of 30% ethanol. This bacteriocin was eluted with a finalwash of 10 ml of 95% ethanol. This active fraction was freeze-driedovernight and resuspended in 0.1% TFA. At each step during thepurification, aliquots of the supernatant, XAD-8 column, cation-exchangecolumn, and resuspended freeze-dried protein fractions were collectedand stored at 4°C for furtheranalysis.

Bacteriocin activity assay. The culture supernatants were assayed for activity against C. divergens LV13 by the spot-on-lawn technique with APT agar.The plates were incubated for 18 h at 30°C. Fractions from theenterocin B purification were assayed by the same method usingMRS agar and L. sake ATCC 20017 as the indicator strain. Activitywas measured by taking the reciprocal of the highest dilutionthat exhibited a clear zone of inhibition and was expressed asAU permilliliter.

MALDI-TOF MS. All mass spectra were acquired on a linear MALDI-TOF mass spectrometer equipped with delayed extraction technology (ProflexIII; Bruker, Billerica, Mass.) with a 125-cm flight tube. Allspectra were acquired in positive ion linear mode with a nitrogenlaser ( $lambda$ = 337 nm) for desorption/ionization of the samples andan acceleration voltage of 20 kV. The spectra are representativeof 60 consecutive laser shots. Angiotensin II (MH⁺ = 1,046.542; Sigma Chemical Co., St. Louis, Mo.) and insulinbovine (MH⁺ = 5,734.557; Sigma) were used as the calibrants for externalmass calibration. The instrument was calibrated for each samplepreparation method by using the conditions describedbelow.

Sample preparation. The use of synthetic membranes and washing the probe with water were examined as methods of removing sample contaminants toprovide effective MALDI-TOF MS analysis. Polyethylene membranes(Fisher Scientific, Fair Lawn, N.J.) were prepared by the methoddescribed by Worral et al. (26). The membrane was saturatedwith methanol, air-dried, and fixed to the stainless steel probewith double-sided tape. Culture supernatant (0.5 µl) was spottedon the membrane and allowed to dry. The membrane was washed threetimes with 20 µl of 70% methanol in water and was air-dried betweeneach set of washes. A saturated solution of sinapinic acid (0.5µl; Sigma) was spotted on the sample. The supernatant of L. lactisATCC 11454 was used to determine the most effective washing methodof the sample directly on the probe (on-target washing). Supernatantsamples (0.5 µl) were placed on a stainless steel MALDI probe,and the probe was allowed to air dry. The probe was dipped intowater and held static for 0, 10, 30, or 60 s. The excess waterwas shaken off, and the probe was air-dried. When dry, 0.5 µlof a saturated solution of sinapinic acid in 0.1% TFA-acetonitrile(2:1) was added to the sample spot and allowed to dry beforeanalysis.

Detection of bacteriocins by bioassay. All supernatants and fractions tested had activity against the appropriate indicator strains (Table 2). The concentrationof bacteriocins in the supernatants varied from 1,600 to 6,400AU/ml when assayed against C. divergens LV13. Throughout the purificationprocedure for enterocin B, the relative AU per milliliter in eachof the fractions increased.

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TABLE 2. Concentrations of bacteriocins in prepared culture supernatants and fractions collected during purification of enterocin B

Detection of bacteriocins by MALDI-TOF MS. Attempts with membranes to adsorb bacteriocins for MALDI-TOF MS analysis were unsuccessful (data not shown). However, theon-target washing method proved to be useful for the detectionof bacteriocins by MALDI-TOF MS. Figure 1A shows the spectrumof the prepared culture supernatant from L. lactis ATCC 11454,which should contain nisin. The natural contaminants in the preparedculture supernatant were present in sufficient concentration toaffect the quality of the protein signal. A 10-s wash with milli-Qwater removed a portion of the contaminants (Fig. 1B); however,a 30-s wash (Fig. 1C) was the most effective in washing away thecontaminants, resulting in a peptide signal of greater intensity,better resolution, and less noise. The 60-s wash (Fig. 1D) wasalso effective in removing the contaminants, but it appeared todegrade the sample signal. Despite poor signal intensity and resolutionfor some of the samples in Fig. 1, the m/z ratios for all sampleswere similar to the mass expected for nisin (MH⁺ = 3,354 ± 0.1%) with signals ranging from 3,355 to 3,359 Da.Similar results were obtained when enterocin B was washed fordifferent times (data not shown). The 30-s wash was used as themethod for sample preparation when attempting to detect otherbacteriocins by MALDI-TOF MS.

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FIG. 1. Comparison of mass spectra obtained from a crude bacteriocin preparation of nisin with either no water rinse (A), a 10-s water rinse (B), a 30-s water rinse (C), or a 60-s water rinse (D).

MALDI-TOF MS was able to detect brochocin A and B, pediocin PA-1, enterocin A, and enterocin B in cell supernatants of theproducer organisms. Figure 2A shows the spectra obtained for theculture supernatant of B. campestris ATCC 43754, which producesbrochocin A (5,242 Da) and brochocin B (3,943 Da) (19). Thepeak in the 2,920-Da range has not been identified. Figure 2Bshows the MALDI-TOF MS spectra obtained from the supernatant ofP. acidilactici PAC-1.0, which produces pediocin PA-1 (4,629 Da)(11). Figures 2C and D are the mass spectra obtained from thesupernatants of E. faecium CTC 492 and E. faecium BFE 900, respectively.E. faecium CTC 492 produces enterocin A, a 47-amino-acid bacteriocinwith a molecular mass of 4,829 Da (2). The MALDI mass spectrumconfirms that E. faecium CTC 492 produced enterocin A, but italso shows another peptide at approximately 5,479 Da, which correspondsto the mass of enterocin B (5,463 Da) (9, 21). E. faeciumCTC 492 also appears to be producing another uncharacterized substance,with a molecular mass of approximately 5,800 Da. The peak at approximately5,479 Da in Fig. 2D confirms that enterocin B is being producedby E. faecium BFE 900.

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FIG. 2. Mass spectra obtained from crude bacteriocin preparations from B. campestris ATCC 43754 (A), P. acidilactici PAC-1.0 (B), E. faecium CTC 492 (C), and E. faecium BFE 900 (D).

MALDI-TOF MS was also effective in determining the presence of bacteriocins in the active fractions obtained during the purificationof enterocin B (Fig. 3). Figure 3A is the MALDI spectrum for thecell supernatant with a small peak at the appropriate mass rangefor enterocin B. The MALDI-TOF MS spectrum for the fraction collectedafter purification on the XAD-8 column (Fig. 3B) also confirmedthe presence of enterocin B. Figure 3C shows that enterocin Aand B were present in the fraction eluted from the cation exchangecolumn. Figure 3D is the MALDI-TOF MS spectrum of the sample afterresuspension of the freeze-dried bacteriocin. Throughout the purification,as the bacteriocin concentration increased, the arbitrary intensityof the peaks increased. However, there does appear to be a slightdiscrepancy in the mass among the samples. Discrepancies betweenthe MALDI-TOF MS mass measurements shown in this figure and thereported masses given in Table 1 could be the result of manyfactors. For example, the mass of enterocin B determined by MALDI-TOFMS (5,479 Da) was 16 Da greater than that reported in the literature.This difference is likely due to oxidation of the peptide. Wanget al. (24) attributed mass discrepancy to difficulty in accuratelydetermining the peak centroid due to the low resolving capabilitiesof MALDI-TOF MS, as well as the use of external versus internalcalibration. External calibration is the method of choice whenspeed and sample consumption rather than mass accuracy are ofinterest. A lower level of mass accuracy is obtained with externalcalibration because slight changes in laser power and sample preparationmay cause differences in the desorption/ionization process. However,an advantage of MALDI-TOF MS is that the results are the averageof many individual laser pulses (23). Therefore, the combinationof a large number of ions and good calibration should alleviateconcern regarding the accuracy of the mass. In this study, itwas shown that MALDI-TOF MS should not be relied upon for an accuratemeasurement of molecular mass; however, it is capable of providingreproducible spectra for the detection of bacteriocins withinthe expected mass range.

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FIG. 3. Mass spectra obtained from fractions of an enterocin B purification supernatant (A), from an XAD-8 column (B), from a cation-exchange column (C), and of resuspended freeze-dried protein (D).

MALDI-TOF MS is the first reported mass spectrometric technique to be used to detect bacteriocins in the cell-free supernatantsof a culture. This is largely due to the ability to purify sampleson target. In our studies, a sterile water wash was chosen asthe method for removing contaminants. Other researchers have suggestedthe use of polyethylene or polypropylene membranes for use asactivated membranes to which the peptide or protein binds (4,5, 26). However, Joosten and Nuñez (15) report that Tween80 prevents adsorption of the bacteriocins nisin and enterocinon polypropylene surfaces. This may explain the loss of peptidesignal found when we studied the use of polyethylene membraneswith various rinses as a sample surface for MALDI-TOF MSanalysis.

The presence of contaminants in the culture supernatant greatly suppresses the signal of the peptide. Blackledge and Alexander(4) suggested that the contaminants prevent effective crystallizationof the matrix and are desorbed with more efficiency than the peptide.This, in turn, suppresses the peptide signal. Amado et al. (1)indicated that the loss of protein signal may be explained bypartial precipitation of surfactant-protein ionic pairs duringsample preparation. They also suggested that the signal degradationfound with high concentrations of surfactants may be the resultof surfactants coating the matrix crystals, thus diminishing energytransfer and desorption/ionization efficiency. The results presentedhere show that a 30-s water rinse in sample preparation removesthe majority of the contaminants, resulting in a better S/N ratio,better peak resolution, and better signal intensity of the samplepeak.

It has also been shown that MALDI-TOF MS can be used to identify components of various samples throughout the bacteriocinpurification process and has potential for future use in the detectionof bacteriocins in genetic and food experiments. Of particularinterest is the potential of MALDI-TOF MS as a quantificationtool. Bouksaïm et al. (6) reported that to use bacteriocinsas food preservatives, it is important to understand the relationshipbetween activity and exact quantity or real concentration of bacteriocinin a food system. However, in order to quantify bacteriocins byMALDI-TOF MS, a pure sample would be needed. The method proposedin this paper for detection would not be very reproducible forquantification given the evidence that spectral changes occurwith washing (Fig. 1). The use of MALDI-TOF MS as a quantitationtool is currently being examined for pure nisin. Purificationmethods for other bacteriocins are being developed, and thesewill be examined by MALDI-TOFMS.

Analysis by MALDI-TOF MS is just beginning to be recognized, and more work is needed in obtaining higher-resolution spectra,better sensitivity, better sample preparation, and faster dataanalysis (1, 7, 23, 26). The results presented hereshow that MALDI-TOF MS is a rapid and sensitive detection methodfor bacteriocins. Its ability to generate mass spectra from thesupernatant makes it particularly attractive for use in industryand commercial application. Another major advantage of MALDI-TOFMS is its ability to screen supernatant and purification samplesfor bacteriocin production. This process takes minimal time (minutes)compared to the overnight incubation of traditional bioassays.Further research will involve the use of MALDI-TOF MS to detectbacteriocins in multicomponent food systems and the examinationof the interaction between the bacteriocins and the differentfoodcomponents.

	ACKNOWLEDGMENTS

This work was supported by grants from the Natural Sciences and Engineering Research Council and the Alberta AgriculturalResearch Institute Farming for the FutureProgram.

We thank Charles Franz, Len Steele, Darcy Driedger, and Jian Wang for their technical assistance andadvice.

	FOOTNOTES

^* Corresponding author. Mailing address: 4-10 Agriculture/Forestry Centre, University of Alberta, Edmonton, Alberta T6G 2P5,Canada. Phone: 780-492-6015. Fax: 780-492-8914. E-mail: lynn.mcmullen{at}ualberta.ca.

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This article has been cited by other articles:

Garneau, S., Ference, C. A., van Belkum, M. J., Stiles, M. E., Vederas, J. C. (2003). Purification and Characterization of Brochocin A and Brochocin B(10-43), a Functional Fragment Generated by Heterologous Expression in Carnobacterium piscicola. Appl. Environ. Microbiol. 69: 1352-1358 [Abstract] [Full Text]
Franz, C. M.�A.�P., Worobo, R. W., Quadri, L. E.�N., Schillinger, U., Holzapfel, W. H., Vederas, J. C., Stiles, M. E. (1999). Atypical Genetic Locus Associated with Constitutive Production of Enterocin B by Enterococcus faecium BFE 900. Appl. Environ. Microbiol. 65: 2170-2178 [Abstract] [Full Text]

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1.	Amado, F. M. L., M. G. Santana-Marques, A. J. Ferrer-Correia, and K. B. Tomer. 1997. Analysis of peptide and protein samples containing surfactants by MALDI-MS. Anal. Chem. 69:1102-1106.
2.	Aymerich, T., H. Holo, L. S. Håvarstein, M. Hugas, M. Garriga, and I. F. Nes. 1996. Biochemical and genetic characterization of enterocin A from Enterococcus faecium, a new antilisterial bacteriocin in the pediocin family of bacteriocins. Appl. Environ. Microbiol. 62:1676-1682[Abstract].
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