Analysis of the Bacteriolytic Enzymes of the Autolytic Lactococcus lactis subsp. cremoris Strain AM2 by Renaturing Polyacrylamide Gel Electrophoresis: Identification of a Prophage-Encoded Enzyme

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Applied and Environmental Microbiology, November 1998, p. 4142-4148, Vol. 64, No. 11
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Analysis of the Bacteriolytic Enzymes of the Autolytic Lactococcus lactis subsp. cremoris Strain AM2 by Renaturing Polyacrylamide Gel Electrophoresis: Identification of a Prophage-Encoded Enzyme

Anne-Sophie Lepeuple, Ellis Van Gemert, and Marie-Pierre Chapot-Chartier^*

Institut National de la Recherche Agronomique, Unité de Recherche de Biochimie et Structure des Proteines, Domaine de Vilvert, 78352 Jouy-en-Josas Cedex, France

Received 22 August 1997/Accepted 11 August 1998

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Lactococcus lactis subsp. cremoris AM2 was previously shown to lyse early and extensively during cheese ripening (M.-P. Chapot-Chartier,C. Deniel, M. Rousseau, L. Vassal, and J.-C. Gripon, Int. DairyJ. 4:251-269, 1994). We analyzed the bacteriolytic activitiesof autolytic strain AM2 by using renaturing sodium dodecyl sulfate-polyacrylamidegel electrophoresis performed with two different substrates inthe gel, Micrococcus lysodeikticus and L. lactis autoclaved cells.Several lytic activities were detected in L. lactis AM2; a majorlytic activity, designated A2 (46 kDa), was found only with theL. lactis cell substrate. This activity appears to be differentfrom major peptidoglycan hydrolase AcmA characterized previously(G. Buist, J. Kok, K. J. Leenhouts, M. Dabrowska, G. Venema, andA. J. Haandrickman, J. Bacteriol. 177:1554-1563, 1995), whichhas a similar molecular mass. The two enzymes differ in substratespecificity as well as in sensitivity to pH and different chemicalcompounds. L. lactis AM2 is lysogenic and mitomycin C inducible.Enzyme A2 was shown to be inducible by mitomycin C and to be prophageencoded. It was identified as an enzyme similar to the lysin encodedby lactococcal small isometric temperate bacteriophages. A prophage-curedderivative of L. lactis AM2 was obtained, and this isolate exhibiteddifferent autolytic properties than AM2. After prolonged incubationin the stationary phase after growth on M17 medium, the extentof lysis of an AM2 culture was 60%, whereas over the same periodthere was almost no lysis in a prophage-cured derivative strainculture. These results suggest that the prophage lytic systemis involved in the strain AM2 lysis observed in liquid mediumand that it could also be involved in the lysis observed duringcheeseripening.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Lactococci, which are widely used as starter bacteria in cheesemaking, participate in the development of cheese flavor throughthe actions of their enzymes (41). Autolysis of these organismsappears to be a crucial step in the release of intracytoplasmicenzymes, such as peptidases that produce free amino acids whichare aroma precursors and degrading hydrophobic peptides whichare responsible for bitter taste. This view is supported by theresults of several experimental studies which correlated enhancementof bacterial lysis with an increase in the free amino acid productionrate and a decrease in bitter taste (3, 4, 9, 10, 21).The autolytic properties of lactococci, which have been studiedin buffer or liquid medium (3, 4, 23, 40) as well asin cheese (8, 43), appear to vary from strain to strain.The following factors could account for the different autolyticbehaviors: the cellular cell wall hydrolase contents, regulationof the expression of the enzymes, and cell wall composition. Anotherpossibility is that a prophage is involved, as previously proposed(12), since numerous strains of lactococci are lysogenic (11).

Bacteria synthesize cell wall hydrolases which are capable of hydrolyzing the peptidoglycan in their own cell envelopes andare also called autolysins. The following four types of enzymesare distinguished on the basis of their cleavage specificities: $beta$ -N-acetylmuramidases (lysozymes), $beta$ -N-acetylglucosaminidases,N-acetylmuramyl-L-alanine amidases, and endopeptidases (37).These enzymes, which are localized in the cell wall and are potentiallylethal to the cells, are synthesized during bacterial growth,and it has been proposed that they are involved in different cellularprocesses, including cell division, cell wall turnover, and transformation.Cell wall hydrolases (lysins) are also encoded by bacteriophageDNA and are synthesized during the bacteriophage lytic cycle.The structural resemblance and potential evolutionary link betweenbacteriophage lysins and bacterial autolysins have been describedpreviously for gram-positive bacteria, such as Streptococcus pneumoniae(14, 15) and Bacillus subtilis (13, 25). In the case ofLactococcus lactis bacteriophages, a second protein, called holin,is required for cell lysis. This protein is a small protein whichis able to make holes in the cytoplasmic membrane and allows thelysin to reach the cell wall peptidoglycan (44).

In previous studies, workers started to evaluate the peptidoglycan hydrolase contents of different L. lactis strains. Therenaturing sodium dodecyl sulfate (SDS)-polyacrylamide gel electrophoresis(PAGE) technique (24, 33), which permits detection of hydrolaseactivity after renaturation in a substrate-containing gel, revealedactivity bands in L. lactis (6, 32, 35). The gene encodingthe major peptidoglycan hydrolase (AcmA) of L. lactis MG1363 hasbeen cloned and sequenced (6). This gene encodes a 46.5-kDaprotein which is probably a muramidase (30), is required forcell separation during growth, and appeared to be present in allof the strainstested.

In a previous study, we compared the autolytic behaviors of two L. lactis starter strains during ripening of pressed-curdcheese (8). We observed that L. lactis subsp. cremoris AM2autolyzes early and extensively, whereas L. lactis subsp. lactisNCDO763 does not autolyze over a period of severalmonths.

In this study, we used the renaturing SDS-PAGE technique to analyze the bacteriolytic activity profile of the autolytic L.lactis strain AM2 and to compare this profile with that of thenonautolytic strain NCDO763 in order to address the question ofthe different autolytic behaviors. In strain AM2 with a lactococcalcell substrate, we detected a major bacteriolytic activity at46 kDa, which was not present in strain NCDO763 or in MG1363 andwas different from the previously described AcmA activity. Wefound that this enzyme was actually encoded by prophage DNA presentin lysogenic strain AM2. We propose that a prophage is involvedin the lysis observed in strain AM2 during cheeseripening.

	MATERIALS AND METHODS

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Bacterial strains and growth conditions. L. lactis strains were obtained from the CNRZ collection (Institut National de la Recherche Agronomique, Jouy-en-Josas, France).The strains were grown at 30°C in M17 broth (39) (Difco Laboratories,Detroit, Mich.) supplemented with 0.5% (wt/vol) lactose (M17-lacbroth); the only exception was strain MG1363, which was grownin M17 broth supplemented with 0.5% (wt/vol) glucose. Growth wasmonitored by measuring the optical density at 650 nm (OD₆₅₀) witha spectrophotometer (model Uvikon 931; Kontron Instruments Inc.,Everett, Mass.).

General DNA techniques. Restriction enzymes were obtained from Boehringer Mannheim and were used as recommended by the supplier. Molecular cloning,purification, and analysis of DNA were performed by using standardprocedures (36). The pBluescript vector was obtained from Stratagene(La Jolla, Calif.).

PCR was carried out by using a model 480 DNA thermal cycler (Perkin-Elmer, Norwalk, Conn.) and Taq DNA polymerase accordingto the instructions of the manufacturer (Oncor, Inc., Gaithersburg,Md.). Primers LYS-1 (5'-ATGAAAAGATTAATCAAAAAATCTG; positions 463to 487) and LYS-2 (5'-TTAATAATTTAGWGTTTGACCAG; positions 1749to 1727) were deduced from the previously published sequence ofthe lysin gene (lys) of lactococcal bacteriophage Tuc2009 (2).Primers PALA-4 (5'-CTTCAACAGACAAGTCC; positions 319 to 335) andPALA-14 (5'-GATAAATGATTCCAAGC; positions 1448 to 1432) correspondedto internal sequences of the acmA gene (6).

Total DNA of L. lactis strains were prepared as previously described (26). They were digested with the appropriate restrictionenzyme (Boehringer Mannheim), electrophoresed in a 0.7% agarosegel, and blotted onto a Hybond-N nylon membrane (Amersham International,Amersham, United Kingdom) by the Southern method as describedby Sambrook et al. (36). Probes corresponding to the fragmentsamplified by PCR performed with the primers described above fromthe total DNA of L. lactis MG1363 (for acmA) or AM2 (for lys)were used as probes for detection of the lys and acmA genes intotal DNA from strains. Labeling of probes and detection wereperformed with an ECL (enhanced chemiluminescence) gene detectionsystem (Amersham) used according to the manufacturer'sinstructions.

DNA sequencing was performed with an ABI PRISM Cycle Sequencing Ready Reaction kit (Perkin-Elmer) used according to the supplier'srecommendations. The DNA sequence was determined with an AppliedBiosystems model 373A automated DNA sequencer (Perkin-Elmer).

SDS-PAGE and renaturing SDS-PAGE. SDS-PAGE was carried out as described by Laemmli (22) with a Mini Protean II cell unit (Bio-Rad Laboratories, Inc., Hercules,Calif.) and a gel that was 75 by 55mm.

Renaturing SDS-PAGE was performed as previously described (24, 33); 0.2% (wt/vol) Micrococcus lysodeikticus ATCC 4698(Sigma Chemicals Co., St. Louis, Mo.) autoclaved cells or 0.4%(wt/vol) L. lactis AM2 autoclaved cells were included in 10 or12% polyacrylamide gels for detection of bacteriolytic activities.Samples were solubilized in sample buffer (62.5 mM Tris-HCl [pH6.8], 2.3% [wt/vol] SDS, 50 mM dithiothreitol [DTT], 10% [vol/vol]glycerol, 0.01% [wt/vol] bromophenol blue) and heated for 3 minat 100°C. When necessary, the sample was centrifuged, and thesoluble material was loaded onto thegel.

After electrophoresis, the gels were washed for 30 min in distilled water at room temperature with gentle shaking, and thenthey were transferred into renaturation buffer containing 50 mMMES (2-morpholinoethanesulfonic acid) (Sigma)-NaOH (pH 6.0) and0.1% (wt/vol) Triton X-100. The gels were incubated with gentleshaking for 16 h at 37°C. They were rinsed with distilled water,stained with 0.1% (wt/vol) methylene blue in 0.01% (wt/vol) KOHfor 2 h at room temperature with gentle shaking (20), and destainedwith distilled water. The bacteriolytic activities appeared asclear bands on a bluebackground.

Molecular masses were determined by comparison with molecular mass standards electrophoresed on the same gel and stained withCoomassie blue (Fast Stain concentrate; Zoion Biotech, Newton,Mass.). The standards were purchased from Bio-Rad Laboratoriesand contained phosphorylase b (molecular weight, 97,400), bovineserum albumin (66,200), ovalbumin (45,000), carbonic anhydrase(31,000), soybean trypsin inhibitor (21,500), and lysozyme (14,400).

The influence of pH and the influence of various chemical compounds on bacteriolytic activities were determined by renaturingSDS-PAGE and incubation of different gel slices in renaturationbuffers containing different compounds. The following bufferswere used to determine the influence of pH: 50 mM sodium acetate(pH 5.0), 50 mM MES-NaOH (pH 6.0), 50 mM Tris-HCl (pH 7.0, 7.5,and 8.0), and 50 mM TAPS [N-tris(Hydroxymethyl)methyl-3-aminopropanesulfonicacid] (Sigma)-NaOH (pH 9.0). In addition, 100 mM NaCl, 100 mMKCl, 10 mM CaCl₂, 10 mM MgCl₂, 10 mM ZnCl₂, 10 mM CuCl₂, 10 mMEDTA, 10 mM iodoacetic acid, and 10 mM DTT were tested by addingthem to renaturation buffer which contained 0.1% Triton X-100.

Preparation of cell extracts and cell wall extracts. L. lactis cells grown in M17 medium were recovered by centrifugation at 8,000 × g for 15 min at 4°C and washed with cold 50mM Tris-HCl (pH 7.0) buffer. Various cell extracts and cell fractionswere prepared as described below in order to determine bacteriolyticactivities by renaturing SDS-PAGE. The culture supernatant wasfiltered through 0.45-µm-pore-size filters (Millex-HA; MilliporeS.A., Bedford, Mass.) and tested for the presence of bacteriolyticactivities.

(i) SDS cell extract. Cells were resuspended in SDS-PAGE sample buffer and heated for 3 min at 100°C, and the insoluble material was removed bycentrifugation at 13,000 × g for 10 min. The supernatant (SDScell extract) was analyzed by renaturing SDS-PAGE.

(ii) LiCl cell extract. The cells from a 100-ml culture were resuspended in 1 ml of a solution containing 50 mM Tris-HCl (pH 7.5), 4 M LiCl, and 1mM phenylmethylsulfonyl fluoride. The suspension was incubatedat 4°C for 30 min. The cells were then removed by centrifugation,and the supernatant was dialyzed against 100 mM LiCl-50 mM Tris-HCl(pH 7.0) and examined by renaturing SDS-PAGE.

(iii) Native cell walls. Native cell walls were prepared after disruption of cells with glass beads. The cells were resuspended in 10 mM sodium phosphatebuffer (pH 7.0) containing 1 mM phenylmethylsulfonyl fluorideand were disrupted with glass beads (diameters, 150 to 212 µm;Sigma) in a bead beater (Vibrogen). The cell walls were recoveredby centrifugation at 25,000 × g for 15 min at 4°C. They were washedtwice with distilled water, twice with 10 mM sodium phosphatebuffer (pH 7.0), and then twice with distilled water again. Thepellet was finally resuspended in distilledwater.

(iv) Cell wall extract and cytoplasmic extract. Spheroplasts were prepared by lysozyme treatment in sucrose-containing buffer as described previously (45). The supernatant(cell wall extract) was recovered. The spheroplast pellet wasresuspended in hypotonic buffer (50 mM Tris-HCl [pH 7.0], 1 mMMgCl₂, 25 U of RNase A [Sigma] per ml, 50 U of DNase I [Sigma]per ml), incubated on ice for 30 min, and centrifuged at 20,000× g for 30 min at 4°C. The supernatant was used as the cytoplasmicextract.

Mitomycin C induction. A 16-h culture was used to inoculate M17-lac broth to an initial OD₆₅₀ of 0.05. The culture was incubated at 30°C until theOD₆₅₀ was 0.3, and mitomycin C (Sigma) was added to a final concentrationof 1 µg/ml as described previously (34). The culture was incubatedfurther at 30°C, and the OD₆₅₀ was monitored regularly. A culturegrown in M17-lac broth at 30°C was used as acontrol.

Preparation and analysis of bacteriophage DNA. A 30-ml M17-lac broth culture of L. lactis AM2 was induced with mitomycin C as described above. After lysis was completed,the lysate was centrifuged at 12,000 × g for 10 min at 15°C toeliminate the cell debris, and the supernatant was filtered througha 0.45-µm-pore-size filter (Millex-HA; Millipore). Bacteriophageparticles were precipitated with polyethylene glycol 4000, andthe phage DNA was extracted as described by Sambrook et al. (36).

Electron microscopy. Fifty milliliters of L. lactis AM2 lysate obtained after mitomycin C induction was centrifuged to eliminate the cell debris.The supernatant was filtered as described above and then centrifugedat 82,000 × g for 2 h at 4°C with an ultracentrifuge (model CentrikonT-1080; Kontron Instruments Inc.). The pellet containing the phageparticles was resuspended in 10 mM Tris-HCl-10 mM MgCl₂ (pH 8.0).The phage particles were stained with 2% uranyl acetate, as previouslydescribed (1), and were observed with a Zeiss model EM-10 electronmicroscope operating at 80kV.

Prophage curing. The method used for prophage curing has been described previously by Gasson and Davies (16). Different dilutions in Ringer'ssolution of an exponential-phase culture (OD₆₅₀, 2.0) were spreadonto M17-lac agar plates and subjected to UV irradiation at awavelength of 310 nm for 5 s with a UV table. The plates wereincubated for 48 h at 30°C shielded from light. A total of 400surviving clones were examined for prophage sensitivity. Theseclones were resuspended in 200 µl of 10% (vol/vol) M17 broth,and single drops (5 µl) of the suspensions were placed onto M17-lacagar plates containing 10 mM calcium chloride that previouslyhad been inoculated with a mitomycin C lysate containing bacteriophageparticles. The plates were incubated at 30°C overnight. Prophage-curedclones were tested to determine their sensitivity to the bacteriophageby determining whether clear zones of lysis were produced in thespot test. However, no sensitive clones were isolated in thisway. Ten clones were then tested to determine their sensitivityto mitomycin C. One of those clones was not inducible, suggestingthat it had lost the prophage. We confirmed that this clone wasa prophage-cured derivative of AM2 (designated AM2-C) by Southernhybridization with a lysin lys geneprobe.

Strain AM2-C was not sensitive to bacteriophage $phi$ AM2 isolated from strain AM2 after mitomycin C induction, as determined bythe double-layer technique (18) or in liquid medium. This couldhave resulted either from a phage defect or from the presenceof another integrated prophage that conferred immunity. In anycase, this explains why during screening for phage sensitivityon agar plates we failed to isolate a cured AM2derivative.

Autolysis in buffer and in M17 broth. Exponential-phase cells (OD₆₅₀, 1.0) grown in M17-lac broth were harvested by centrifugation at 8,000 × g for 10 min at 4°C.The pellet was washed in 50 mM sodium acetate buffer (pH 5.0),50 mM MES-NaOH buffer (pH 6.0), or 50 mM sodium phosphate buffer(pH 7.0). The cells were resuspended in the same buffer to aninitial OD₆₀₀ of 0.7. The cell suspensions were incubated at 30°C,and autolysis was monitored by determining the decrease in OD₆₀₀.The extent of autolysis was expressed as the percent decreasein OD₆₀₀ after sometime.

The autolysis of stationary-phase cells in M17 broth at 30°C over a several-day period was monitored by determining the changein OD₆₅₀. Cell viability was determined after the cells were platedonto M17 agar plates and incubated for 48 h at 30°C. The releaseof X-prolyl-dipeptidyl aminopeptidase (PepX) was monitored bymeasuring the enzymatic activity in the culture supernatant withthe Ala-Pro-paranitroanilide (Bachem, Bubendorf, Switzerland)substrate as described by Zevaco et al. (45). The activity unitused was the katal (1 kat of enzyme activity released 1 mol ofparanitroaniline pers).

	RESULTS

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Detection of the bacteriolytic activities of the autolytic strain L. lactis subsp. cremoris AM2 by renaturing SDS-PAGE. L. lactis subsp. cremoris AM2 was described previously as an autolytic strain during cheese ripening (8). We analyzed thebacteriolytic activities of strain AM2 by the renaturing SDS-PAGEtechnique and compared these activities to the activities of L.lactis subsp. lactis NCDO763, which has been described as a nonautolyticstrain (8), and L. lactis subsp. cremoris MG1363, which exhibitsa major AcmA autolysin cloned and sequenced previously (6).Two different substrates were included in the gel, autoclavedM. lysodeikticus and L. lactis cells. The presence of enzymaticactivities was first determined with SDS cell extracts obtainedfrom the three strains grown in M17medium.

With the M. lysodeikticus substrate, no activity band was detected in the strain AM2 SDS cell extract (Fig. 1A, lane 3). Underthe same conditions, the activity profiles obtained with L. lactisNCDO763 and MG1363 were consistent with the results of a previousstudy (6), and the following three activity bands were identified(Fig. 1A, lanes 1 and 2): band B1, a major band at 45 kDa whichcorresponded to major peptidoglycan hydrolase AcmA; band B0, aminor band at 50 kDa which was found to be a precursor of AcmA(6); and band B2, a minor band at 38 kDa which was probablya degradation product of AcmA (6).

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FIG. 1. Detection of bacteriolytic activities of L. lactis MG1363, NCDO763, and AM2 by renaturing SDS-PAGE. (A) Gel containing autoclaved M. lysodeikticus cells as the substrate. (B) Gel containing autoclaved L. lactis cells as the substrate. Lane 1, MG1363 SDS cell extract; lane 2, NCDO763 SDS cell extract; lane 3, AM2 SDS cell extract. The positions of the lytic bands are indicated by arrowheads. The numbers on the left are molecular masses (in kilodaltons).

With the L. lactis substrate under the same conditions, three activity bands were detected in AM2, major band A2 (46 kDa)and minor bands A1 (50 kDa) and A3 (34 kDa) (Fig. 1B, lane 3).Detection of the minor bands varied from one experiment to another.For strains NCDO763 and MG1363 (Fig. 1B, lanes 1 and 2), bandB1 was detected, but the band intensity was lower than the bandintensity on the micrococcus substrate, as previously reported(6, 32).

Thus, the major bacteriolytic activity detected in L. lactis AM2, A2 activity, appears to be different from AcmA; the twoactivities differ in substrate specificity, and the A2 activityhas a slightly higher molecular weight thanAcmA.

Despite the fact that AcmA activity was not detected in the SDS cell extract of L. lactis AM2, the presence of the acmA genein AM2 total DNA was shown by the results of PCR amplificationwith specific primers derived from the acmA sequence and by Southernhybridization (data not shown). Total DNA digests from L. lactisAM2 and MG1363 were probed with the acmA PCR product. The acmAgene was found to reside on a 2.5-kb EcoRV fragment (data notshown). In addition, AcmA activity was detected in a native cellwall preparation obtained from L. lactis AM2 when M. lysodeikticuswas the substrate (Fig. 2). These results suggest that the amountof autolysin AcmA in strain AM2 is lower than the amounts of AcmAin other strains or that it is more difficult to extract AcmAfrom strain AM2 than from other strains because of differencesin the cell envelope structure.

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FIG. 2. Detection of bacteriolytic activities of L. lactis NCDO763 and AM2 by renaturing SDS-PAGE in a gel containing autoclaved M. lysodeikticus cells as the substrate. Lane 1, native cell wall preparation from strain AM2; lane 2, NCDO763 SDS cell extract. The positions of the lytic bands are indicated by arrowheads.

Different cell extracts and fractions (native cell wall, cell wall extract prepared with lysozyme, cytoplasmic fraction, LiClcell extract) of strains AM2 and NCDO763 were prepared and testedto determine whether there were extra bacteriolytic activitiesin gels containing micrococci or lactococci, but no extra lyticactivity was detected (data not shown). When the cells were harvestedat different times during cell growth, no extra bands were observedin the activityprofiles.

The effects of the renaturing buffer pH on the two main activities, A2 and AcmA, were studied by incubating gel slices indifferent buffer solutions. The optimum pH for A2 activity rangedfrom 5.0 to 6.0, whereas the optimum pH for AcmA activity rangedfrom 6.0 to 7.0. The effects of different cations and chemicalcompounds on the A2 and AcmA activities were also examined. Theintensity of the AcmA activity band was enhanced by Ca²⁺, Mg²⁺, and Mn²⁺ and was decreased by Cu²⁺. A2 activity was inhibited by Cu²⁺ and was partially inhibited by Zn²⁺. EDTA, DTT, and iodoacetic acid had no effect on eitheractivity.

The differences in the optimal pH values and sensitivities to some cations between the AcmA and A2 activities and the differencesin substrate specificities and molecular masses strongly suggestedthat these activities correspond to two different bacteriolyticenzymes.

Identification of the major bacteriolytic activity detected in L. lactis subsp. cremoris AM2 as a mitomycin C-inducible lytic enzyme. Numerous L. lactis strains have been found to be lysogenic, and the majority of them can be induced by treatment with mitomycinC (11). An exponentially growing culture of strain AM2 (OD₆₅₀,0.3) was exposed to mitomycin C (1 µg/ml). Two hours after theaddition of mitomycin C, growth was arrested and the culture lysed,which resulted in a decrease in the OD₆₅₀ to a value close tothe initial value (Fig. 3A).

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FIG. 3. Effect of mitomycin C on the growth of L. lactis subsp. cremoris AM2 (A) and on its bacteriolytic activity profile (B and C). (A) Symbols: $black-triangle$ , untreated culture; $bullet$ , mitomycin C induction. The arrow indicates the time of mitomycin C (1 µg/ml) addition. (B and C) Samples were removed at 1-h intervals from the untreated culture (B) or from the mitomycin C-induced culture (C), and SDS cell extracts containing the same amount of proteins were analyzed by renaturing SDS-PAGE. Lanes 1 through 6, samples taken at zero time and at 1, 2, 3, 4, and 5 h after mitomycin C addition. The position of lytic band A2 is indicated by an arrowhead.

Electron microscopy of the AM2 lysate revealed the presence of a multitude of intact bacteriophage particles (Fig. 4), confirmingthat strain AM2 is lysogenic. A single kind of particles was present;each particle had a small isometric head, a noncontractile tail,and a base plate. The tail was about 120 nm long, and the headwas about 44 nm in diameter. To characterize the bacteriophageliberated (designated $phi$ AM2), the phage DNA was extracted and digestedwith EcoRI (data not shown). The sum of the sizes of all of theresulting fragments was about 43 kb; these fragments probablyrepresented the genome of a single lactococcal bacteriophage (19).

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FIG. 4. Electron micrograph of bacteriophage particles observed in an L. lactis AM2 lysate after mitomycin C induction. Bar = 50 nm.

During mitomycin C induction of L. lactis AM2, samples were removed at 1-h intervals, and the corresponding SDS cell extractswere prepared and analyzed by renaturing SDS-PAGE; the same amountof protein was placed in each well. Two hours after the additionof mitomycin C, the intensity of the A2 activity in the gel increasedsignificantly (Fig. 3C), and it remained high over the next 3h, during which cellular lysis took place. A concomitant increasein the A2 activity was observed in the culture supernatant (datanot shown). In the control culture not treated with mitomycinC, the intensity of the A2 activity did not vary in this way duringgrowth for the same period of time (Fig. 3B). Thus, major bacteriolyticenzyme A2 detected in AM2 appears to be mitomycin C inducible.This suggests that it is encoded by prophageDNA.

In order to confirm that the A2 enzyme was prophage encoded, a derivative of L. lactis AM2 cured of its prophage (designatedstrain AM2-C) was obtained as described in Materials and Methods.The bacteriolytic activities present in strain AM2-C were thendetermined by renaturing SDS-PAGE after preparation of an SDScell extract. With the lactococcal substrate, A2 activity wasnot present in strain AM2-C, and only one of the weaker activitybands that detected in AM2, band A1 was present (Fig. 5). Withthe micrococcal substrate, as observed for strain AM2, no activitywas detected in strain AM2-C (data not shown), although the acmAgene was detected in AM2-C total DNA by Southern hybridizationwith a 2.5-kb EcoRV fragment, as observed for strains AM2 andMG1363 (data not shown). These results confirmed that the majorbacteriolytic activity detected in L. lactis AM2, A2 activity,is prophage encoded.

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FIG. 5. Bacteriolytic activity profile of prophage-cured derivative AM2-C of L. lactis AM2 as determined by renaturing SDS-PAGE performed with a gel containing autoclaved L. lactis cells as the substrate. Lane 1, AM2 SDS cell extract; lane 2, AM2-C SDS cell extract. The same amount of proteins was loaded into each well.

Identification of the major bacteriolytic enzyme detected in L. lactis AM2. Several lysin genes of bacteriophages that infect L. lactis have been cloned and sequenced previously. Four different typesof lysins, which do not exhibit sequence similarity to each other,have been characterized (17). One of these lysins, the lysinencoded by small isometric temperate bacteriophages Tuc2009 (2)and $phi$ LC3 (5), has a molecular mass of 46,000 Da, which is closeto the molecular mass of the A2 lytic activity described above.Thus, we examined whether A2 could be identical to this enzyme.Using oligonucleotide primers corresponding to the 5' and 3' endsof the lysin structural gene (lys), we performed tests to determinethe presence of the lysin gene in $phi$ AM2 bacteriophage DNA and inAM2 total DNA by PCR amplification. A DNA fragment that was 1.2kb long (the expected size of the lysin gene) was amplified fromboth DNA templates. As a control for bacteriophage DNA purity,we verified that the lactococcal pepX gene (28, 31) couldbe amplified from AM2 total DNA but not from the bacteriophageDNA (data not shown). The lysin PCR amplification product wasused to probe total DNA digests from both L. lactis AM2 and AM2-Cand bacteriophage $phi$ AM2. The lys gene was found to reside on a7.3-kb ClaI fragment in $phi$ AM2 and AM2 DNA but was not detectedin AM2-C DNA, confirming that AM2-C was a bacteriophage $phi$ AM2-curedderivative of AM2 (Fig. 6). In addition, the probe hybridizedwith a second fragment which was larger than 9 kb, indicatingthat strains AM2 and AM2-C could contain another prophage thathad a homologous lysin gene and was not inducible by mitomycinC. After being cloned in the E. coli pBluescript plasmid vector,the PCR amplification product was sequenced. The nucleotide sequenceconfirmed that the amplified gene was identical to the lysin lysgene.

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FIG. 6. Southern blot hybridization analysis of total DNA from different strains and bacteriophage $phi$ AM2. Lane 1, L. lactis subsp. cremoris AM2; lane 2, L. lactis subsp. cremoris AM2-C; lane 3, bacteriophage $phi$ AM2. DNA was cut with ClaI and hybridized with the 1.2-kb lys PCR product as the probe. The numbers on the left indicate molecular sizes (in kilobases).

Thus, the major bacteriolytic activity detected in strain AM2, A2 activity, is prophage encoded and is similar to the 46-kDalysin previously identified in small isometric temperate bacteriophagesTuc2009 and $phi$ LC3.

Growth characteristics and temperature sensitivity of L. lactis AM2 and its prophage-cured derivative. L. lactis AM2 was previously described as a temperature-sensitive strain, and it was postulated that the thermosensitivityof this organism results from induction of a thermoinducible prophage(12). Therefore, we examined whether the prophage-cured derivativeobtained in this study, strain AM2-C, was sensitive totemperature.

In M17-lac broth, strains AM2 and AM2-C grew at the same rate at each temperature tested (30, 33, and 35°C) and did not growat 37 and 40°C (data notshown).

The effect of a temperature shift to 40°C during growth at 30°C was then tested. The strains were grown in M17-lac broth at30°C to an OD₆₅₀ of 0.25, 0.3, or 0.5, and the cultures were subsequentlyshifted to 40°C. The two strains exhibited the same initial growthrate, followed by growth inhibition about 2 h after the temperatureshift. A portion of the culture (about 25%) lysed after the growthinhibition (data not shown). Thus, prophage-cured derivative strainAM2-C was still temperature sensitive. The temperature sensitivityof the two strains could be attributed to the presence of a secondprophage.

The only difference which was observed between the two strains grown in M17 medium was the fact that a strain AM2-C culturesedimented more rapidly than strain AM2 and produced cell aggregates,although the chains were notlonger.

Autolytic properties of L. lactis AM2 and its prophage-cured derivative. Exponential-phase cells of L. lactis AM2 and AM2-C were resuspended in buffers at different pH values between 5 and 7 andincubated at 30°C. Then lysis was monitored by determining thedecrease in OD₆₀₀ during a 24-h period. No differences in theautolytic properties of AM2 and AM2-C were detected (results notshown).

Strains AM2 and AM2-C were grown in M17-lac medium and then were incubated after they reached the stationary phase for severaldays at 30°C. Lysis was monitored by determining the change inthe OD₆₅₀ of each culture, as well as the release into the culturesupernatant of PepX, which was used as an intracytoplasmic marker(38); cell viability was determined on agar plates at 1-dayintervals (Fig. 7). In both cases, the viable cell populationdecreased rapidly between the first day and the third day. Incontrast, only the OD₆₅₀ of the AM2 culture decreased rapidlybetween the fourth day and the sixth day before it stabilizedat a value which was around 40% of the initial OD₆₅₀ value. TheOD₆₅₀ of the AM2-C culture remained constant over a 9-day period.For strain AM2, we observed that the decrease in OD₆₅₀ was accompaniedby a concomitant release of PepX activity into the culture supernatant.In contrast, no PepX activity was detected in the strain AM2-Cculture supernatant. These results confirmed that the decreasein OD₆₅₀ reflected cell lysis and the release of the intracytoplasmiccontents.

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FIG. 7. Autolysis after prolonged incubation in the stationary phase after growth in M17-lac broth at 30°C of L. lactis subsp. cremoris AM2 (A) and L. lactis subsp. cremoris AM2-C (B). Bacterial lysis was monitored by determining the changes in broth turbidity ( $bullet$ ) (expressed as percentages of the maximum OD₆₅₀), in cell viability ( $open circle$ ) (expressed as percentages of the maximum number of CFU per milliliter), and in the PepX activity released into the culture supernatant ( $black-triangle$ ) (expressed in nanokatals per milliliter of culture supernatant). PepX activity was measured with Ala-Pro-paranitroanilide as the substrate. Similar results were obtained in three independent experiments.

Previously, the lysis of an L. lactis culture observed after it reaches the stationary phase has been attributed to activityof the major autolysin, AcmA (7). Thus, the slow rate of autolysisduring the beginning the stationary phase observed for strainsAM2 and AM2-C could be related to the low amounts of AcmA detectedin the two strains. In contrast, the lysis of the AM2 culture,but not the AM2-C culture, observed after several days could berelated to the presence of the A2 bacteriolytic activity in theAM2culture.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Using the renaturing SDS-PAGE technique, we evaluated the bacteriolytic activities of L. lactis subsp. cremoris AM2, a strainpreviously reported to autolyze during cheese ripening when itwas used as a starter strain (8). The enzymatic activity profileof strain AM2 varied according to the substrate included in thegel (that is, M. lysodeikticus or L. lactis cells). Previously,M. lysodeikticus has been reported to allow more sensitive detectionof lytic activities by several authors (24, 32). However,in the case of strain AM2, the use of L. lactis cells as the substrateallowed detection of three bacteriolytic activities which werenot detected with micrococci, including a major activity, theA2 activity (46 kDa). All of these activities differ from thepreviously detected activities, as determined by renaturing SDS-PAGE.The AcmA major peptidoglycan hydrolase (6) appears to be presentin strain AM2 but at a lower level than in the other strains tested.Major bacteriolytic enzyme A2 detected in strain AM2 was clearlydistinct from AcmA on the basis of differences in substrate specificity,molecular mass, optimal pH, and sensitivity to different divalentcations.

According to our results, the major A2 enzyme detected in L. lactis AM2 by renaturing SDS-PAGE is not an autolysin but isencoded by prophage DNA present in lysogenic strain AM2. We identifiedthe A2 enzyme as an enzyme which was similar to the lysin of Tuc2009(2) and $phi$ LC3 (5), which are small isometric temperate bacteriophageswhose lys gene was previously cloned and sequenced. This lysinis a 429-amino acid protein which has an N-terminal catalyticdomain and a C-terminal domain containing two highly homologoussequence repeats of 43 amino acids which are presumably involvedin binding and recognition of the cell wall substrate (5).

Detection of prophage-associated lytic activities by the renaturing SDS-PAGE technique was reported previously for Bacillussubtilis prophages (13, 25). However, in contrast to the A2activity, these lytic activities produced weak bands comparedto the bands corresponding toautolysins.

The presence of the A2 activity in the AM2 activity electrophoretic profile did not result from induction of the prophageafter cells were harvested and washed during preparation of cellextracts, since when the washing step was omitted, the band wasstill detected and it had the same intensity. This indicates thatthe A2 enzyme is present in the cells or at least a portion ofthe cells during the growth in M17 medium. Spontaneous inductionof bacteriophages from lysogenic L. lactis strains grown on M17medium has been described previously (34), and this could accountfor the detection of the A2 activityband.

We compared the autolytic properties of L. lactis AM2 and its prophage-cured derivative, AM2-C. These two strains differ inthe ability to lyse during prolonged incubation in the stationaryphase after growth on M17 medium, suggesting that the prophagelytic enzyme A2 may play a role in the lysis observed. Since prophageinduction is likely to happen only in growing cells, lysis probablyresults from the A2 activity that accumulates in a portion ofthe cells. This enzyme, which is synthesized without a signalsequence (2, 5), cannot be transported through the cytoplasmicmembrane. Thus, it requires the action of a holin also encodedby the prophage to make holes in the cell membrane or permeabilizationof the cytoplasmic membrane under starvationconditions.

It has been proposed previously that a prophage is involved in the lysis of L. lactis starter strains observed in cheese (12,29). The previous studies described temperature-sensitive strainsthat exhibited thermoinducible lysis when they were subjectedto a temperature shift similar to the one used in the manufactureof cheddar cheese, and the authors attributed this property toinduction of a prophage. The prophage identified in the presentstudy does not seem to be involved in the thermosensitivity ofL. lactis AM2. In addition, we previously observed lysis of L.lactis AM2 in pressed-curd cheese manufactured without a temperatureshift (8). Nevertheless, the possibility that the bacteriophagelytic enzyme which we identified is involved in the early lysisof L. lactis AM2 in cheese is supported by several observations.First, there appears to be a lower amount of the AcmA major autolysinin strain AM2 than in other L. lactis strains, especially strainNCDO763, which was found to be nonautolytic in cheese. Second,strain AM2 and its prophage-cured derivative differ in the autolyticproperties studied after prolonged incubation in M17 medium inthe stationary phase. Third, A2 activity was detected especiallyin strains that were previously described as nonbitter strainsor strains in which there was a rapid decrease in cell viabilityin cheese trials (12, 27, 42, 43) (unpublished data).Further comparisons in cheese assays of strain AM2 and its prophage-curedderivative when they are used as starter strains should allowus to clarify the role of the prophage lytic proteins in the lysisof AM2 observed incheese.

	ACKNOWLEDGMENTS

We are very grateful to M.-C. Chopin for helpful advice and discussions and to J.-C. Gripon for his continued interest inthis work. We warmly thank B. Cesselin for the electron microscopyobservations and B. Nicolas and P. Regent for photographicwork.

	FOOTNOTES

^* Corresponding author. Mailing address: INRA, Unité de Recherche de Biochimie et Structure des Proteines Domaine de Vilvert,78352 Jouy-en-Josas Cedex, France. Phone: 01 34 65 22 68. Fax:01 34 65 21 63. E-mail: chapot{at}biotec.inra.jouy.fr.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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1.	Accolas, J.-P., and H. Spillmann. 1979. The morphology of six bacteriophages of Streptococcus thermophilus. J. Appl. Bacteriol. 47:135-144.
2.	Arendt, E.-K., C. Daly, G. F. Fitzgerald, and M. Van de Guchte. 1994. Molecular characterization of lactococcal bacteriophage Tuc2009 and identification and analysis of genes encoding lysin, a putative holin, and two structural proteins. Appl. Environ. Microbiol. 60:1875-1883[Abstract/Free Full Text].
3.	Bie, R., and G. Sjöström. 1975. Autolytic properties of some lactic acid bacteria used in cheese production. Part I. Material and methods. Milchwissenschaft 30:653-657.
4.	Bie, R., and G. Sjöström. 1975. Autolytic properties of some lactic acid bacteria used in cheese production. Part II. Experiments with fluid substrates and cheese. Milchwissenschaft 30:739-747.
5.	Birkeland, N.-K. 1994. Cloning, molecular characterization, and expression of the genes encoding the lytic functions of lactococcal bacteriophage $phi$ LC3: a dual lysis system of modular design. Can. J. Microbiol. 40:658-665[Medline].
6.	Buist, G., J. Kok, J. Leenhouts, M. Dabrowska, G. Venema, and A. J. Haandrikman. 1995. Molecular cloning and nucleotide sequence of the gene encoding the major peptidoglycan hydrolase of Lactococcus lactis, a muramidase needed for cell separation. J. Bacteriol. 177:1554-1563[Abstract/Free Full Text].
7.	Buist, G., H. Karsens, A. Nauta, D. van Sinderen, G. Venema, and J. Kok. 1997. Autolysis of Lactococcus lactis caused by induced overproduction of its major autolysin, AcmA. Appl. Environ. Microbiol. 63:2722-2728[Abstract/Free Full Text].
8.	Chapot-Chartier, M.-P., C. Deniel, M. Rousseau, L. Vassal, and J.-C. Gripon. 1994. Autolysis of two strains of Lactococcus lactis during cheese ripening. Int. Dairy J. 4:251-269.
9.	Crow, V. L., F. G. Martley, T. Coolbear, and S. J. Roundhill. 1995. The influence of phage-assisted lysis of Lactococcus lactis subsp. lactis ML8 on Cheddar cheese ripening. Int. Dairy J. 5:451-472.
10.	Crow, V. L., T. Coolbear, F. G. Gopal, F. G. Martley, L. L. McKay, and H. Riepe. 1995. The role of autolysis of lactic acid bacteria in the ripening of cheese. Int. Dairy J. 5:855-875.
11.	Davidson, B. E., I. B. Powell, and A. J. Hillier. 1990. Temperate bacteriophages and lysogeny in lactic acid bacteria. FEMS Microbiol. Rev. 87:79-90.
12.	Feirtag, J. M., and L. McKay. 1987. Thermoinducible lysis of temperature-sensitive Streptococcus cremoris strains. J. Dairy Sci. 70:1779-1784[Abstract/Free Full Text].
13.	Foster, S. J. 1993. Analysis of Bacillus subtilis 168 prophage-associated lytic enzymes: identification and characterization of CWLA-related prophage proteins. J. Gen. Microbiol. 139:3177-3184[Abstract/Free Full Text].
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