Cloning and Characterization of the Genes Encoding a Cytochrome P450 (PipA) Involved in Piperidine and Pyrrolidine Utilization and Its Regulatory Protein (PipR) in Mycobacterium smegmatis mc2155

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Journal of Bacteriology, June 1999, p. 3419-3426, Vol. 181, No. 11
0021-9193/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Cloning and Characterization of the Genes Encoding a Cytochrome P450 (PipA) Involved in Piperidine and Pyrrolidine Utilization and Its Regulatory Protein (PipR) in Mycobacterium smegmatis mc²155

Pascal Poupin, Véronique Ducrocq, Sylvie Hallier-Soulier, and Nicole Truffaut^*

Laboratoire de Génétique Microbienne, Université de Technologie de Compiègne, Centre de Recherches, 60205 Compiègne, France

Received 21 December 1998/Accepted 6 April 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods References

Transposon mutagenesis of Mycobacterium smegmatis mc²155 enabled the isolation of a mutant strain (called LGM1) altered inthe regulation of piperidine and pyrrolidine utilization. Thecomplete nucleotide sequence of the gene inactivated in mutantLGM1 was determined from the wild-type strain. This gene (pipR)encoded a member of the GntR family of bacterial regulatory proteins.An insertion element (IS1096), previously described for M. smegmatis,was detected downstream of the gene pipR. Three additional openreading frames were found downstream of IS1096. The first openreading frame (pipA) appeared to encode a protein identified asa cytochrome P450 enzyme. This gene is the first member of a newfamily, CYP151. By a gene replacement experiment, it was demonstratedthat the cytochrome P450 pipA gene is required for piperidineand pyrrolidine utilization in M. smegmatis mc²155. Genes homologous to pipA were detected by hybridization inseveral, previously isolated, morpholine-degrading mycobacterialstrains. A gene encoding a putative [3Fe-4S] ferredoxin (orf1)and a truncated gene encoding a putative glutamine synthetase(orf2') were found downstream of pipA.

	INTRODUCTION

Top Abstract Introduction Materials and Methods References

Rapidly growing species of the genus Mycobacterium play an important role in the metabolism of a variety of recalcitrant organicmolecules, including vinyl chloride (20), polycyclic aromatichydrocarbons (6, 14, 24, 26), halogenated phenols (52,53), isonicotinate (30), aromatic compounds (10, 45, 48,50), and secondary amines (8, 11, 28, 29, 40). Morpholine,pyrrolidine, and piperidine are closely related secondary aminesused in industry and eventually released in the environment. Thelatter two compounds can also be synthesized by different organisms.Recently, we isolated several mycobacterial strains able to degrademorpholine and demonstrated that a cytochrome P450 enzyme wasinvolved in the degradation of this amine in all these strains(41). All these bacteria, like nearly all the morpholine degradersdescribed in the literature, belong to the genus Mycobacterium.The induction of a heme-containing monooxygenase was also notedwhen these bacteria were grown on pyrrolidine and, for some ofthem, on piperidine. It was shown that morpholine-nondegradingmycobacterial strains (Mycobacterium fortuitum and Mycobacteriumsmegmatis mc²155) produced a cytochrome P450 monooxygenase during growth onpiperidine and pyrrolidine (41).

Cytochromes P450 are heme-containing enzymes which play a central role in the oxidative metabolism of organic compounds. Theseproteins seem to be important for mycobacteria, since 22 genesencoding putative cytochromes P450 have been detected in the genomeof Mycobacterium tuberculosis (13).

In this study, we have isolated, sequenced, and analyzed the genes encoding the piperidine-inducible cytochrome P450 (PipA)and its regulatory protein (PipR) from the M. smegmatis strainmc²155. The isolation of a mutant, in which pipR was inactivatedby transposition mutagenesis, clearly demonstrated the involvementof the protein PipR in the regulation of piperidine and pyrrolidinemetabolism. It was shown, by gene replacement experiment, thatpipA was required for piperidine and pyrrolidine utilization instrain mc²155.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods References

Bacterial strains, plasmids, and growth conditions. The bacterial strains and plasmids used in this study are listed in Table 1. Escherichia coli was grown in liquid mediumor on solid Luria-Bertani (L) medium containing ampicillin (50µg ml¹), gentamicin (20 µg ml¹), kanamycin (20 µg ml¹), or streptomycin (50 µg ml¹). M. smegmatis mc²155 was grown in Middlebrook liquid 7H9 medium or solid 7H10 medium(Difco, Fisher Scientific, Elancourt, France) supplemented withBacto Middlebrook ADC Enrichment supplement and 0.05% Tween 80,at 37°C except for transposition mutagenesis. With this strain,gentamicin and kanamycin were used at 5 and 20 µg per ml, respectively.Other mycobacterial strains were grown in liquid medium or onsolid L medium at 30°C.

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TABLE 1. Bacterial strains and plasmids used

In gene replacement experiments, transformants were selected on solid L medium containing gentamicin and kanamycin (LGK).Ten percent sucrose was added to solid L medium containing kanamycin(LKS) to select allelic-exchangeevents.

Mineral salts (MS) medium which contained (per liter) 1 g of KH₂PO₄, 1 g of K₂HPO₄, 0.04 g of MgSO₄ · 7H₂O, 0.004 g of FeCl₃· 6H₂O, and 1 g of (NH₄)₂SO₄ (the last compound was omitted whenthe amines were used as the carbon, nitrogen, and energy sources)was used to grow mycobacterial strains on piperidine, pyrrolidine,or glucose. Noble agar (Difco) was added at 1.5% (wt/vol) to preparesolid MS medium. The pH was adjusted to 7.0 with HCl after theaddition of the amine. Piperidine (C₅H₁₁N) and pyrrolidine (C₄H₉N)were purchased from Fluka (Sigma Aldrich Sarl, St. Quentin Fallavier,France) and used at 10 mM. Bacterial growth was determined bymonitoring the optical density of the cultures at 600nm.

Degradation of piperidine and pyrrolidine by M. smegmatis resting cells. Cells growing in 7H9 medium or MS medium amended with piperidine were harvested, at the end of the exponential phase, by centrifugationat 6,000 × g for 10 min at 20°C. The supernatant was discarded,and the pellet was washed twice with MS medium and resuspendedin 8 ml of this medium (circa 10¹⁰ cells per ml). Cells were incubated with 5 mM piperidine or pyrrolidineat 37°C with magnetic agitation and aeration (2 liters of airper h). Samples (110 µl) were taken at regular intervals and immediatelycentrifuged at 20,000 × g for 2 min, and the concentration ofthe amine wasdetermined.

Analytical methods. The piperidine and pyrrolidine concentrations were estimated spectrophotometrically by the method of Stevens and Skov (49)as modified by Knapp et al. (28). The protein concentrationwas determined by the method of Bradford (7).

Spectrophotometric analysis of cytochrome P450. Glucose-grown M. smegmatis cells were harvested by centrifugation (6,000 × g for 10 min) at 4°C. Cells were broken by threepassages through a French pressure cell (SLM-Aminco) at 18,000lb in². The crude extract was treated as previously described (40).

DNA manipulations. Restriction and modification enzymes were purchased from Eurogentec (Eurogentec S.A., Seraing, Belgium). Plasmid DNA isolationwas performed with a Qiagen plasmid extraction kit (Qiagen S.A.,Courtaboeuf, France). DNA fragments of interest were purifiedfrom agarose gel by using the Geneclean III kit (Bio 101, Ozyme,St. Quentin, France). Standard recombinant DNA techniques werecarried out as described by Sambrook et al. (43).

Electroporation of bacteria. Electrocompetent E. coli cells were prepared and electroporated by the method of Dower et al. (17). Cells of M. smegmatismc²155 were made electrocompetent and used according to the methoddescribed by Pelicic et al. (38).

Tn611 transposon mutagenesis. The transposon mutagenesis of M. smegmatis mc²155 was performed as described by Guilhot et al. (19) by using the thermosensitiveplasmid pCG79. This vector, carrying Tn611, was introduced intoM. smegmatis by electroporation, and transformants were selectedon 7H10 medium containing kanamycin at 30°C. A randomly chosenclone was grown for 72 h at 30°C in 5 ml of 7H9 medium supplementedwith kanamycin. Antibiotic-free 7H9 medium was then inoculatedwith this preculture and incubated for 24 h at 39°C. Various dilutionswere spread on 7H10 medium supplemented with kanamycin and incubatedat 39°C. Eight thousand clones were taken at random and replicaplated on solid MS medium containing 10 mM piperidine plus kanamycinand on 7H10 medium containingkanamycin.

Isolation of genomic DNA, gene cloning, and sequencing. M. smegmatis genomic DNA was isolated from a 10-ml culture (7H9 medium) as follows. Cells were pelleted by centrifugation(6,000 × g for 10 min), resuspended in 5 ml of 7H9 medium supplementedwith 50 µg of D-cycloserine ml¹ and 100 µg of lysozyme ml¹, and incubated overnight at 37°C. After centrifugation, the cellswere resuspended in 500 µl of solution I (25% glucose, 50 mM Tris-HCl[pH 8.0], 50 mM EDTA, 500 µg of lysozyme ml¹) and incubated for 1 h at 37°C. Then, 500 µl of solution II (100mM Tris-HCl [pH 8.0], 50 mM EDTA, 400 µg of proteinase K ml¹) was added and the mixture was incubated for 3 h at 55°C. DNAwas extracted twice with phenol-chloroform and once with chloroformand then was ethanol precipitated. The pellet was dissolved in1× TE buffer (10 mM Tris-HCl [pH 8.0], 1 mM EDTA) and treatedwith RNase A (50 µg ml¹) for 1 h at 37°C. Proteinase K (50 µg ml¹) was added to the DNA solution, and incubation was continuedfor 1 h at 37°C. DNA was extracted with phenol-chloroform andchloroform and then concentrated by ethanol precipitation. Thegenomic DNA of the other mycobacterial strains was isolated aspreviously described (41).

The site of the Tn611 insertion in the chromosome of mutant LGM1 was determined by using marker rescue as described by Billman-Jacobeet al. (5). Genomic DNA of strain LGM1 was digested with therestriction enzyme EcoRI (a unique site in pCG79), diluted, self-ligated,and transformed into E. coli. Transformants were selected on solidL medium supplemented with streptomycin and checked for theirability to grow in kanamycin-containing medium. An EcoRI-HindIIIDNA fragment (759 bp) of M. smegmatis chromosomal origin was subclonedinto pBluescript II KS(+) (Stratagene, Ozyme, St. Quentin, France)for sequence analysis. The HindIII restriction site is situatedin IS6100a (position 3,300) of Tn610 (GenBank accession no. X53635).Tn611 is a derivative of Tn610 in which the sulfonamide resistance(sul3) gene has been replaced by the Km resistance (Km^r) gene of Tn903 (31). The 759-bp DNA fragment was used in hybridizationexperiments (probe I). Total DNA of wild-type M. smegmatis mc²155 was digested overnight with different restriction endonucleasesand separated by electrophoresis by using a 0.8% agarose gel.Southern blots (neutral membrane; Appligene Oncor, Illkirch, France)were hybridized with the digoxigenin-labeled probes. The labelingmethod, prehybridization and hybridization steps, and detectionprocedure were performed as recommended by the manufacturer (BoehringerMannheim S.A., Meylan, France). Prehybridization and hybridizationwere performed at 42°C by using 50% formamide in solutions. DNAfragments of interest were purified from the agarose gel and clonedinto pBluescript II KS(+). Double-stranded DNA sequencing wascarried out with an automated sequencer (Genome Express, Paris,France). The French server BISANCE (15) was used to performcomputer-assisted sequence analyses. The homologies between oursequences and the database sequences were determined by usingthe FASTA (36) and BLASTP (1)programs.

Construction of pLGM23. The plasmid pLGM21 was linearized with the restriction enzyme MluI (which acts on a single site in the pipA gene), treatedwith Klenow fragment to fill in the ends of the restriction site,and ligated to a blunt-ended PstI fragment (approximately 1.1kb) containing the Tn903 Km^r cassette (aph) to obtain the pLGM22 vector. A 2.8-kb XbaI-PstIfragment containing the pipA::Km region of plasmid pLGM22 wasblunt ended and ligated into the SmaI site in pJQ200 to generatethe suicide vector pLGM23 (Table 1).

Nucleotide sequence accession numbers. The nucleotide sequences presented in this study have been assigned accession no. AF102509 and AF102510 byGenBank.

	RESULTS AND DISCUSSION

Pyrrolidine and piperidine utilization by M. smegmatis mc²155. M. smegmatis mc²155 is able to grow in liquid MS medium containing piperidine or pyrrolidine as the sole sources of carbon,nitrogen, and energy. Piperidine and pyrrolidine were degradedquite rapidly, and after 80 h of incubation, no secondary aminescould be detected in the culture medium. The values for turbidityof the cultures increased from 0.02 to 1.00 and 0.84 in piperidine-containingmedium and pyrrolidine-containing medium, respectively (data notshown).

Isolation and characterization of a transposon-induced piperidine utilization mutant of M. smegmatis mc²155. In order to isolate M. smegmatis mutants altered in piperidine metabolism, Tn611 transposon mutagenesis was performed as describedby Guilhot et al. (19). A total of 8,000 thermoresistant clonesrandomly selected from the library were replica plated on MS agarmedium containing 10 mM piperidine and on 7H10 medium. Both typesof medium were supplemented with kanamycin. After five days ofincubation at 39°C on piperidine-containing MS agar medium, acolony growing faster than other ones was obtained. This clone(called strain LGM1) was isolated for furtheranalysis.

The kinetics of piperidine and pyrrolidine degradation by M. smegmatis mc²155 and strain LGM1 resting cells were determined (data not shown).When mc²155 cells were grown in MS medium containing piperidine, the degradationof this amine began rapidly. All of this compound disappearedfrom the medium within 60 min. Over the same period, the degradationof piperidine by M. smegmatis mc²155 cells grown in 7H9 medium was very slow. The results are consistentwith the fact that the piperidine degradation pathway of strainmc²155 is inducible. In contrast, cells of strain LGM1 pregrown in7H9 medium could degrade piperidine and pyrrolidine with the sameefficiency as piperidine-grown mc²155 cells. The enzymes associated with the ability to degradepiperidine and pyrrolidine in M. smegmatis mc²155 need not be induced in strainLGM1.

A spectrophotometric analysis of reduced extracts of mycobacterial cells (strains mc²155 and LGM1) grown in MS medium supplemented with glucose wasrecorded. In the spectrum of CO-treated minus nontreated reducedextracts of strain LGM1 cells, an absorption maximum at about450 nm was observed, indicating the presence of a cytochrome P450(Fig. 1). This peak was not detected in strain mc²155 cell extracts. Extracts prepared from glucose-grown LGM1 cells,piperidine-grown LGM1 cells, and piperidine-grown strain mc²155 cells all contained similar amounts of cytochrome P450 (125pmol per mg of protein). Thus, a constitutive expression of acytochrome P450 in mutant LGM1 was noted. This monooxygenase couldcorrespond to the cytochrome P450 involved in the metabolism ofpiperidine in M. smegmatis mc²155. Therefore, a gene encoding a protein involved in the negativeregulation of the synthesis of this cytochrome P450 was probablydisrupted by the insertion of Tn611.

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FIG. 1. Reduced CO difference spectra of crude extracts of glucose-grown M. smegmatis cells. Spectrum a, Tn611 insertion mutant LGM1; spectrum b, wild-type, M. smegmatis mc²155 strain. The protein concentrations were 10 mg ml¹.

Site of insertion of transposon Tn611 in strain LGM1. Tn611 has been shown to transpose by a replicative mechanism (31). During this transposition event, plasmid pCG79 containingTn611 was integrated into the chromosome of the bacteria and oneof the two copies of IS6100 was duplicated. Thus, by digestingthe genomic DNA of the Tn611 insertional mutant bacteria by EcoRI(which acts on a unique site in pCG79) it was possible to rescuea plasmid containing the origin of replication for pUC18 and theStr^r and/or the Km^r markers (depending on which IS6100 copy was duplicated). Therescued plasmid obtained after strain LGM1 genomic DNA digestionwith the restriction endonuclease EcoRI was introduced into E.coli. This plasmid conferred only Str^r to E. coli. Consequently, during the process of transpositionof Tn611 in M. smegmatis IS6100a was duplicated since the rescuedplasmid obtained after IS6100b duplication would have conferredStr^r plus Km^r to E. coli. The DNA sequence of chromosomal origin was subclonedfrom the rescued plasmid and sequenced on one strand (data notshown). In this nucleotide sequence, 737 bp belong to M. smegmatisgenomic DNA and 22 bp belong to IS6100a of transposon Tn611. Thededuced polypeptide had similarity to proteins of the GntR familyof bacterial regulatory proteins (21).

Cloning of the gene encoding a regulatory protein of the piperidine metabolism pathway. The 737-bp fragment from M. smegmatis LGM1 chromosome (probe I) was used to probe Southern blots of completely digested M.smegmatis mc²155 DNA in order to isolate the entire gene. An EcoRI fragmentof about 5.8 kb was detected, cloned in pBluescript II KS(+) (pLGM20),and selected by colony hybridization. Southern blot hybridizationanalysis of plasmid pLGM20 DNA, digested with several restrictionendonucleases, was carried out with probe I (data not shown).The gene encoding the regulatory protein was located on one endof the 5.8-kb EcoRI fragment (Fig. 2). Starting from this end,a 1,215-bp region was sequenced on both strands. Sequence analysisof this DNA fragment revealed the presence of an open readingframe (ORF) (designated pipR) encoding a protein of 245 aminoacids with a calculated molecular mass of 26,331 Da (Fig. 3).This ORF begins with a GUG initiation codon, is preceded by thesequence AAGGAG, a putative ribosome binding site, and is followedby a sequence potentially forming a stable transcription terminationhairpin structure. The use of GUG as the translational initiationcodon of PipR could allow the autoregulation of the expressionof this protein as demonstrated for the cam repressor (CamR) ofthe cytochrome P-450cam hydrolase operon (2). The pipR-encodedprotein shows significant similarity to members of the GntR bacterialregulatory family, as follows: a probable transcriptional regulator(SCI35_36) of Streptomyces coelicolor (35) (31% identity in234 amino acids), a putative lactate operon regulator (LctR) ofE. coli (16) (30% identity in 227 amino acids), a pyruvate dehydrogenasecomplex repressor (PdhR) of Rhodobacter capsulatus (54) (28%identity in 218 amino acids), and an Uxu operon regulator (UxuR)of Haemophilus influenzae (18) (27% identity in 238 amino acids).In members of this family (21), a conserved helix-turn-helixDNA-binding domain was found in the N-terminal part of the protein([LIVAPKR]-[PILV]-X- [EQTIVMR]-X₂-[LIVM]-X₃-[LIVFT]-[DNGSTK]-[RGTLV]-X-[STAIVP]-[LIVA]-X₂-[STAGV]-[LIVMFYH]-X₂-[LMA]). This PROSITE(3) consensus sequence (PROSITE accession no. PS00043) wasdetected in the N-terminal region of PipR protein, between residues38 and 62, but with two differences, at positions 51 (A insteadof [DNGSTK]) and 52 (P instead of [RGTLV]). Many members of thisfamily act as transcriptional repressors and possess, in additionto the DNA-binding domain, an effector-binding domain.

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FIG. 2. Map of the 5.8-kb EcoRI DNA region of M. smegmatis mc²155 containing the piperidine-inducible cytochrome P450 (pipA) and its regulatory gene (pipR). The DNA regions sequenced on both strands are indicated in shaded boxes. The other ORFs shown correspond to the putative resolvase (TnpR) and transposase (TnpA) of IS1096 insertion element and to the putative ferredoxin (ORF1) and glutamine synthetase (truncated ORF2') of M. smegmatis mc²155. Only the restriction sites mentioned in the text are indicated. The position of Tn611 insertion (triangle) into the pipR gene, determined from sequence analysis, is shown.

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FIG. 3. Nucleotide sequence of the 1,215-bp fragment containing the regulatory protein (PipR) gene. The presumptive ribosome binding site aaggaaga (italic), the stop codon (asterisk), and the nucleotides potentially involved in the formation of a stem-loop structure (underlined) are indicated. The GenBank accession number is AF102509. Bases shown in lowercase letters are noncoding sequences.

Identification of putative functional ORFs. The DNA sequence downstream of pipR was partially sequenced (data not shown). It is identical to the nucleic acid sequenceencoding the putative resolvase of the insertion element IS1096(GenBank accession no. M76495) isolated from M. smegmatis mc²6 by Cirillo et al. (12). This insertion element is 2,276 bpin length. Strain mc²155 is an efficient plasmid transformation mutant of M. smegmatismc²6.

The 2,177-bp SacI-EcoRI fragment located downstream of IS1096 was subcloned (pLGM21), and its nucleotide sequence was determined(Fig. 4). In this sequence, three ORFs (designated pipA, orf1,and orf2') were found in the same orientation. The last ORF (orf2')was truncated. The deduced amino acid sequence of pipA (400 aminoacids; M_r, 44,747) matches the PROSITE consensus motif, F-[SGNH]-X-[GD]-X-[RHPT]-X-C-[LIMVFAP]-[GAD],for cytochromes P450 (PROSITE accession no. PS00086). PipA showssimilarity to bacterial cytochromes P450, as follows: 31% identityto a putative cytochrome P450 (MTV023_25) of M. tuberculosis (13),31% identity to a cytochrome P450-like protein governing hydroxylationand epoxidation in mycinamicin II biosynthesis of Micromonosporagriseorubida (22), and 36% identity (but in a 291-amino-acidoverlap only) to a cytochrome P450 of Streptomyces hygroscopicus(32). PipA clearly has less than 40% identity with known P450proteins, which indicates that it represents the first memberof a new family, CYP151 (33). Upstream of pipA, two imperfectrepeats, which could constitute a DNA-binding motif, were detected.An imperfect 9-bp inverted repeat sequence spanned the putative $-$ 35 region (TTGACA) of pipA, and a 7-bp imperfect inverted repeatwas localized between the putative $-$ 10 region (TAGAGT) and theputative ribosome binding site (GGAGG) of pipA. Bacterial cytochromesP450 are often substrate inducible, and the expression of someof them has been shown to be negatively regulated at a transcriptionallevel. The expression of the cytochrome P450_BM-3 gene of Bacillusmegaterium ATCC 14581 (46) and of the cytochrome P-450cam ofPseudomonas putida PpG1 ATCC 17543 (2) were demonstrated tobe negatively regulated through the interaction of a repressorwith an operator (inverted repeats) located upstream of thesegenes. In both these cases, the genes encoding cytochrome P450and their regulatory proteins were adjacent and divergently oriented.

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FIG. 4. Nucleotide sequence of the 2,177-bp SacI-EcoRI region encoding a cytochrome P450 (PipA), a putative ferredoxin (ORF1), and a putative glutamine synthetase (truncated ORF2'). The two sets of possible inverted repeats (underlined) in the putative promoter region of pipA, the putative ribosome binding sites ggagg (italic), and stop codons (asterisks) are indicated. The first 182 nucleotides of this sequence are identical to the end of the IS1096 insertion element (positions 2086 to 2268) except for one nucleotide: the base A, in position 2147 in IS1096, is missing. The GenBank accession number is AF102510. Bases shown in lowercase letters are noncoding sequences.

The presence of sequences homologous to the M. smegmatis pipA gene was checked, with the internal PvuI fragment of pipA (788bp) used as a probe (probe II), in the genomes of the followingmycobacterial strains: Mycobacterium sp. strains BM01, BM04, BM05,BM06, FM10, FM30, LM20, LM32, LM40, and RP1 and Mycobacteriumaurum MO1. These different strains were isolated from activatedsludge, soils, or sediments for their ability to degrade morpholine(11, 40, 41). They are also able to degrade pyrrolidineand eventually piperidine. The degradation of these cyclic aminesrequired the involvement of a cytochrome P450 in all these bacteria.A positive signal was obtained with all the DNAs tested in theexperiment, indicating that closely related cytochrome P450 genesare present in these strains (data not shown). The bacteria testedin this study are not representative of all the rapidly growingmycobacterial strains but represent several clusters as definedby the phylogenetic analysis of Pitulle et al. (39). Thus, itis tempting to conclude that a homologous gene encoding a cytochromeP450 involved in the metabolism of cyclic amines is present inrapidly growingmycobacteria.

An ORF encoding a protein of 62 amino acids with an M_r of 6,760 (orf1) was identified in the region downstream of pipA. ThisORF begins 46 bp after the stop codon (UGA) of pipA. The two genesare in the same reading frame. The amino acid sequence of theprotein was 44, 41, and 40% identical to the reported primarystructures of ferredoxin 2 and ferredoxin 1 (Fd-1 and Fd-2) fromStreptomyces griseolus (34) and a putative ferredoxin (AE001094_1)from Archaeoglobus fulgidus (27), respectively. As shown inFig. 5, the three cysteine residues (Cys-11, Cys-17, and Cys-56of Fd-1 and Cys-10, Cys-16, and Cys-55 of Fd-2) supposed to beinvolved in ligating a [3Fe-4S] cluster in each of Fd-1 and Fd-2(34) are conserved in the protein encoded by orf1 (Cys-10, Cys-16,and Cys-53). Type II cytochrome P450 systems, which are foundin bacteria, use a flavin-containing reductase and a small iron-and sulfur-containing redox protein (ferredoxin) to transfer electronsto the terminal cytochrome P450. However, no ferredoxin reductasegene was detected downstream of pipA. In the genome of M. tuberculosis(13), two genes encoding putative ferredoxin proteins (MTCY369_08cand MTV049_08) linked to cytochrome P450 genes (MTCY369_09c andMTV049_07c) were found. The sequences of these ferredoxins aresimilar to that of the ferredoxin of M. smegmatis. The cytochromeP450 systems cloned from S. griseolus (34) and Streptomycesgriseus (51) contain a cytochrome P450 gene and, downstream,the ferredoxin one. Cytochrome P450 systems present in Streptomycesand Mycobacterium strains are similarly organized.

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FIG. 5. Amino acid sequence comparisons of S. griseolus (Fd-1 and Fd-2) and M. smegmatis (Fdpip) ferredoxins. The three cysteine residues, which are supposed to be involved in the attachment of a [3Fe-4S] cluster and are conserved in all three proteins, are indicated in bold. Hyphens indicate gaps introduced to optimize alignments. Residues that are identical in at least two of the three sequences are boxed.

A truncated ORF (orf2') was detected, on the SacI-EcoRI DNA sequence, 6 bp downstream of the UGA stop codon of orf1. The polypeptidededuced from this incomplete gene shows significant homology withdifferent glutamine synthetases (GlnA) from Archaea and Eubacteria.It is 28, 31, and 24% identical to the putative GlnA (U67574_10)of Methanococcus jannaschii (9), the putative GlnA (MTV003_4)of M. tuberculosis (13), and the GlnA (SSGLNA_2) of Sulfolobussolfataricus (44), respectively. Glutamine synthetase catalyzesthe formation of glutamine by condensation of glutamate and ammoniaand therefore plays a key role in the metabolism of nitrogen.A consensus pattern, [FYWL]-D-G-S-S-X_6,8-[DENQSTAK]-[SA]-[DE]-X₂-[LIVMFY],is usually present in the N-terminal section of these enzymes(PROSITE accession no. PS00180). The putative GlnA of M. jannaschiiand the GlnA of S. solfataricus contain this consensus sequence,but it is missing in the putative GlnA of M. tuberculosis andM. smegmatis mc²155. The three ORFs (pipA, orf1, and orf2') are closely linkedand could form part of anoperon.

Disruption of the pipA gene. Experiments were performed to replace the functional allele pipA with an inactivated copy (pipA::Km) in M. smegmatis mc²155. A two-step method for gene replacement, as described by Pelicicet al. (38), was performed by using the suicide vector pLGM23and M. smegmatis mc²155. This plasmid carries the aacC1 and sacB genes, from the pJQ200vector (42), which confer to mycobacteria gentamicin resistanceand sucrose sensitivity, respectively (37). An individual clonewas randomly chosen from those obtained on LGK plates, was propagatedovernight in 7H9 medium containing kanamycin, and was spread onLKS plates. The clones resulting from this experiment were expectedto contain the interrupted allele of the pipA gene. A Southernblot analysis was performed on 10 randomly chosen clones by usingprobe II (data not shown). The internal pipA probe hybridizedto a 3.9-kb fragment of the PstI-digested DNA of M. smegmatismc²155, as expected. All the clones selected on medium containingkanamycin plus sucrose showed hybridization to a 5-kb fragment.An additional hybridization fragment was observed in one clone(clone 4) which could have been the result of a single recombinationevent in the pipA gene. The plasmid pLGM23 was still present inthe chromosome of this bacterium, since this clone was resistantto gentamicin. The resistance to sucrose could be due to a mutationin sacB gene. All these clones showed a shift in the size of thefragment hybridizing to the internal pipA probe (from 3.9 to 5kb) corresponding to the length of the aph cassette. The abilityof these clones to grow on piperidine- or pyrrolidine-containingMS medium or to degrade these compounds was tested. None of thesebacteria could grow on these amines or degrade them (data notshown). These results clearly indicated the involvement of CYP151in the piperidine and pyrrolidine degradative pathway. However,growth was noted in piperidine- and pyrrolidine-containing mediumwith clone 4 when incubation had been prolonged for several days.The interrupted allele of the pipA gene could have been eliminatedby a deletion-recombination event in some bacteria of thisclone.

The cytochrome P450 PipA could catalyze the C-N bond cleavage of piperidine and pyrrolidine rings, as has been suggested formorpholine metabolism by Mycobacterium sp. strain RP1 (40),but further experiments have to be done to confirm this. Jacobyand Fredericks (23) have studied the metabolism of pyrrolidineby Pseudomonas fluorescens ATCC 13430. No pyrrolidine-induciblecytochrome P450 was described for this strain, but it is worthnoting that their experiments were done in 1959. The authors proposeda pathway for pyrrolidine deg-radation (pyrrolidine $right-arrow$ $Delta$ ¹-pyrrolidine $right-arrow$ $gamma$ -aminobutyralde-hyde $right-arrow$ $gamma$ -aminobutyric acid $right-arrow$ succinicacid semialdehyde $right-arrow$ succinate) by this strain. They demonstratedthat the enzymes induced by pyrrolidine metabolism were also detectedduring putrescine utilization. The linearized compounds formedduring piperidine or pyrrolidine metabolism by M. smegmatis mc²155 could be further transformed by enzymes involved in the cadaverineor putrescine utilizationpathways.

Cytochromes P450 have been shown to play a central role in many anabolic and catabolic reactions performed by bacteria, particularlyby actinomycetes. Among rapidly growing mycobacteria, the cytochromeP450 systems induced in Mycobacterium chlorophenolicum by pentachlorophenol(53), in M. fortuitum CG-2 by halogenated phenols (52), andin M. fortuitum KCTC 1062 by steroids (25) have not yet beengenetically characterized. At least 20 cytochrome P-450 geneswere found in the genome of M. tuberculosis (13). The physiologicalfunction of these proteins is still unknown, but one of them (CYP51-likeP450) was able to convert, in vitro, dihydrolanosterol to its14 $alpha$ -demethylated product (4). Some of these cytochrome P450enzymes could be involved in the synthesis of the complex cellwall components and therefore could constitute potential targetsfor antimycobacterialdrugs.

	ACKNOWLEDGMENTS

We thank S. N. Snapper and W. R. Jacobs for the gift of M. smegmatis mc²155, C. Guilhot and B. Gicquel for supplying plasmids pCG79 andpJQ200, and J. S. Cech for providing M. aurumMO1.

	FOOTNOTES

^* Corresponding author. Mailing address: Laboratoire de Génétique Microbienne, Université de Technologie de Compiègne, B.P.20529, 60205 Compiègne, France. Phone: 33 3 44 23 44 52. Fax:33 3 44 20 48 13. E-mail: nicole.truffaut{at}utc.fr.

Present address: Marine Biotechnology Institute, 3-75-1 Heita, Kamaishi, Iwate 026,Japan.

Present address: CIRSEE, 78230 Le Pecq,France.

REFERENCES

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Abstract
Introduction
Materials and Methods
References

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	ALL ASM JOURNALS

1.	Altschul, S. F., W. Gish, W. Miller, E. W. Myersand, and D. J. Lipman. 1990. Basic local alignment search tool. J. Mol. Biol. 215:403-410[Medline].
2.	Aramaki, H., Y. Sagara, H. Kabata, N. Shimamoto, and T. Horiuchi. 1995. Purification and characterization of a cam repressor (CamR) for the cytochrome P-450cam hydroxylase operon on the Pseudomonas putida CAM plasmid. J. Bacteriol. 177:3120-3127[Abstract/Free Full Text].
3.	Bairoch, A. 1992. PROSITE: a dictionary of sites and patterns in proteins. Nucleic Acids Res. 20:2013-2018.
4.	Bellamine, A., A. T. Mangla, D. Nes, and M. R. Waterman. 1998. Is the Mycobacterium tuberculosis CYP51-like P450 a 14 $alpha$ -demethylase?, abstr. IC-11. In F. Durst, and S. L. Kelly (ed.), Program and abstracts of the Fourth International Symposium on P450 Biodiversity and Biotechnology, Strasbourg, France.
5.	Billman-Jacobe, H., J. Sloan, and R. L. Coppel. 1996. Analysis of isoniazid-resistant transposon mutants of Mycobacterium smegmatis. FEMS Microbiol. Lett. 144:47-52[Medline].
6.	Boldrin, B., A. Tiehm, and C. Fritzsche. 1993. Degradation of phenanthrene, fluorene, fluoranthene, and pyrene by a Mycobacterium sp. Appl. Environ. Microbiol. 59:1927-1930[Abstract/Free Full Text].
7.	Bradford, M. M. 1976. A rapid and sensitive method for the quantitation of microgram quantities of protein utilizing the principle of protein-dye binding. Anal. Biochem. 72:248-254[Medline].
8.	Brown, V. R., and J. S. Knapp. 1990. The effect of withdrawal of morpholine from the influent and its reinstatement on the performance and microbial ecology of a model activated sludge plant treating a morpholine-containing influent. J. Appl. Microbiol. 69:43-53.
9.	Bult, C. J., O. White, G. J. Olsen, L. Zhou, R. D. Fleischmann, G. G. Sutton, J. A. Blake, L. M. FitzGerald, R. A. Clayton, J. D. Gocayne, A. R. Kerlavage, B. A. Dougherty, J. Tomb, M. D. Adams, C. I. Reich, R. Overbeek, E. F. Kirkness, K. G. Weinstock, J. M. Merrick, A. Glodek, J. D. Scott, N. S. Geoghagen, J. F. Weidman, J. L. Fuhrmann, D. T. Nguyen, T. Utterback, J. M. Kelley, J. D. Peterson, P. W. Sadow, M. C. Hanna, M. D. Cotton, M. A. Hurst, K. M. Roberts, B. B. Kaine, M. Borodovsky, H. P. Klenk, C. M. Fraser, H. O. Smith, C. R. Woese, and J. C. Venter. 1996. Complete genome sequence of the methanogenic archaeon, Methanococcus jannaschii. Science 273:1058-1073[Abstract].
10.	Burback, B. L., and J. J. Perry. 1993. Biodegradation and biotransformation of groundwater pollutant mixtures by Mycobacterium vaccae. Appl. Environ. Microbiol. 59:1025-1029[Abstract/Free Full Text].
11.	Cech, J. S., P. Hartman, M. Slosarek, and J. Chudoba. 1988. Isolation and identification of a morpholine-degrading bacterium. Appl. Environ. Microbiol. 54:619-621[Abstract/Free Full Text].
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