Identification and targeted disruption of the gene encoding the main 3-ketosteroid dehydrogenase in Mycobacterium smegmatis
Anna Brzostek1,
Tomasz
liwi
ski2,
Anna Rumijowska-Galewicz1,
Ma
gorzata Korycka-Macha
a1 and
Jaros
aw Dziadek1
1 Medical Biology Centre, Polish Academy of Sciences, Lodowa 106, 93-232
odz, Poland
2 Department of Biotechnology and Food Science, Technical University of
odz, Wolczanska 171/173, 90-924
odz, Poland
Correspondence
Jaros
aw Dziadek
jdziadek{at}cbm.pan.pl
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ABSTRACT
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The catabolic potential for sterol degradation of fast-growing mycobacteria is well known. However, no genes or enzymes responsible for the steroid degradation process have been identified as yet in these species. One of the key enzymes required for degradation of the steroid ring structure is 3-ketosteroid
1-dehydrogenase (KsdD). The recent annotation of the Mycobacterium smegmatis genome (TIGR database) revealed six KsdD homologues. Targeted disruption of the MSMEG5898 (ksdD-1) gene, but not the MSMEG4855 (ksdD-2) gene, resulted in partial inactivation of the cholesterol degradation pathway and accumulation of the intermediate 4-androstene-3,17-dione. This effect was reversible by the introduction of the wild-type ksdD-1 gene into M. smegmatis
ksdD-1 or overexpression of ksdD-2. The data indicate that KsdD1 is the main KsdD in M. smegmatis, but that KsdD2 is able to perform the cholesterol degradation process when overproduced.
Abbreviations: 9OHAD, 9
-hydroxy-4-androstene-3,17-dione; AD, 4-androstene-3,17-dione; ADD, 1,4-androstadiene-3,17-dione; DCO, double-crossover homologous recombinant; Kan, kanamycin; KsdD, 3-ketosteroid
1-dehydrogenase; SCO, single-crossover homologous recombinant
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INTRODUCTION
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It has been known since the 1960s that fast-growing mycobacteria degrade natural sterols and use them as a source of carbon and energy. A number of Mycobacterium strains treated with mutagens have been reported to accumulate sterol biodegradation intermediates such as 4-androstene-3,17-dione (AD) and 1,4-androstadiene-3,17-dione (ADD) (Mahato & Garai, 1997
; Martin, 1977
; Szentirmai, 1990
). These intermediates may be used as precursors for the production of steroid drugs and hormones (Sedlaczek, 1988
). Two enzymes, 3-ketosteroid
1-dehydrogenase (KsdD) and 3-ketosteroid 9
-hydroxylase (KsdH) are essential to initiate steroid ring degradation (Fig. 1
). KsdD catalyses transhydrogenation of 3-keto-4-ene-steroid to 3-keto-1,4-diene-steroid, e.g. progesterone to ADD. ksdD genes have been isolated and overproduced from a number of micro-organisms (Molnar et al., 1995
; Choi et al., 1995
; Itagaki et al., 1990
; Kaufmann et al., 1992
; Morii et al., 1998
), but the most abundant data about enzymes involved in steroid skeleton degradation have come from the study of Comamonas testosteroni (Plesiat et al., 1991
; Florin et al., 1996
; Horinouchi et al., 2001
, 2003a
, b
). The inactivation of KsdD may lead to the accumulation of 9
-hydroxy-4-androstene-3,17-dione (9OHAD) from steroid compounds.
Studies on Rhodococcus erythropolis KstD show two distinct enzymes with KsdD activity (Geize et al., 2000
, 2001
). The disruption of both genes was required to block effectively the AD degradation process (Geize et al., 2002
). Reported mycobacterial activities in sterol biodegradation (Wilmanska et al., 1995
; Wovcha et al., 1979
) are not supported by the identification and molecular characterization of genes involved in this process. Here we report on the identification of the main ksdD gene in Mycobacterium smegmatis and its characterization by unmarked gene deletion.
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METHODS
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Bacterial strains and culture conditions.
The following bacterial strains were used: Escherichia coli Top10 (Invitrogen), Mycobacterium smegmatis mc2155 (Snapper et al., 1990
) and Mycobacterium tuberculosis H37Ra. The mycobacterial strains were cultured in Middlebrook 7H9 broth or 7H10 agar plates supplemented with albumin-glucose and 25 µg kanamycin (Kan) ml1 (when required). For steroid bioconversion experiments, mycobacterial strains were cultured in NB broth [8·0 g nutrient broth (Difco) l1, 10·0 g glucose l1, supplemented with 0·2 % Tween 80 (pH 6·06·2)] or in mineral medium [g l1: MgSO4.7H2O, 0·5; Na2HPO4, 1·0; KH2PO4, 0·5; NH4NO3, 2·5; CaCl2.2H2O, 0·001; Fe2(SO4)3.nH2O, 0·01; MnSO4.nH2O, 0·0001; Co(NO3)2.6H2O, 0·000005; (NH4)6Mo7O24.4H2O, 0·0001].
Plasmid constructions.
The plasmid DNA of mycobacterial transformants was recovered and analysed as described by Madiraju et al. (2000)
.
Standard molecular biology protocols were used for this purpose (Sambrook et al., 1989
). All PCR products were obtained using thermostable ExTaq polymerase (Takara) and were cloned initially into a TA vector (pGemTeasy; Promega), then released by digestion with appropriate restriction enzymes before cloning into expression vectors. To facilitate subcloning into expression vectors, restriction enzyme recognition sites (underlined, see below) were incorporated into the sequence of the primers. The plasmids used in this work are listed in Table 1
.
Gene replacement constructs.
To perform unmarked deletions in ksdD-1 and ksdD-2 genes of M. smegmatis, suicidal recombination delivery vectors were constructed. In the first step the 5' ends of the ksdD genes (40 bp ksdD-1; 19 bp ksdD-2) and upstream regions were amplified using primers MsD1GR1 (5'-AACTGCAGGGATTCCGGATCGATGCCG-3') and MsD1GR2 (5'-CCAAGCTTCGCTCCCGACCACCACAAG-3') for ksdD-1, and MsD2GR1 (5'-CCCAAGCTTCCATGATGTCACTCATCGCG-3') and MsD2GR2 (5'-CGGGATCCCGAAGGAGTCGTGGAGGCCG-3') for ksdD-2, and cloned into the PstI/HindIII and HindIII/BamHI sites of p2NIL to create pTS6 and pAB44, respectively. Subsequently, the 3' ends of the ksdD genes (418 bp ksdD-1; 1008 bp ksdD-2) and downstream regions were amplified using primers MsD1GR3 (5'-CCAAGCTTGAAGACCGGCCTGCCCGCCG-3') and MsD1GR4 (5'-CGGGATCCCGCGCGGTTACGCCGGGACC-3') for ksdD-1, and MsD2GR3 (5'-CGGGATCCGTCACCTCGGCACGCGCGG-3') and MsD2GR4 (5'-TGCCGCCCACGACGAGTGCGG-3') for ksdD-2, and cloned into the HindIII/BamHI sites of pTS8 and BamHI/KpnI sites of pAB45. The ligated 5' and 3' fragments of the ksdD-1 and ksdD-2 genes in the resulting vectors were out of frame. Finally, a 6 kb PacI marker cassette from pGOAL17 carrying lacZ and sacB genes was cloned into the PacI site of pTS8 and pAB45 to create pTS10 and pAB46, respectively.
Complementation and overexpression constructs.
Two ORFs (MSMEG5898, ksdD-1; MSMEG4855, ksdD-2) were PCR-amplified using primers MsD1s (5'-GGAAGATCTATGACTGGACAGGAGTACG-3') and MsD1r (5'-GCTCTAGAGCCCTTCCGGGAGGCCGC-3') for ksdD-1, and MsD2s (5'-GAAGATCTATGACTGATTCGAACGGCCTCC-3') and MsD2r (5'-GCTCTAGATTATCAGTCGACTGATTTGCCCG-3') for ksdD-2, and cloned into the BamHI/XbaI sites of pJam2 downstream from the Pami promoter. The resulting constructs carrying putative M. smegmatis ksdD-1 and ksdD-2 genes were named pTS1 and pAB42, respectively. The putative ksdD genes of M. tuberculosis were PCR-amplified using TbD1s (5'-GAAGATCTATGACTGTGCAGGAGTTCG-3') and TbD1r (5'-GGAATTCTCAGCGCTTTCCCGCATGATCG-3') for ksdD-1tb (MT3641) or TbD2s (5'-CGGGATCCGTGGCGTTAACCTGTACCG-3') and TbD2r (5'-CCCAAGCTTCTAGCGGATATCCTCGGCGGC-3') for ksdD-2tb (MT0809). The PCR products were cloned into the BamHI/EcoRI (ksdD-1tb) or BamHI/HindIII (ksdD-2tb) sites of pMV261 under control of the Phsp promoter. The resulting constructs carrying ksdD-1tb or ksdD-2tb were named pAB49 and pAB43, respectively.
Disruption of ksdD-1 and ksdD-2 genes.
The protocol of Parish & Stoker (2000)
was used to disrupt ksdD-1, ksdD-2 or both genes at their native loci on the chromosome. Plasmid DNA (pTS10, pAB46) was treated with NaOH (0·2 mM) and integrated into the M. smegmatis mc2155 chromosome by homologous recombination. The resulting single-crossover homologous recombinant (SCO) mutant colonies were blue, KanR and sensitive to sucrose. The site of recombination was confirmed by PCR and Southern hybridization. The SCO strains were further processed to select for double-crossover (DCO) mutants that were white, KanS and resistant to sucrose (2 %). PCR and Southern hybridization were used to distinguish between the wild-type and DCO mutants.
Steroid standards.
-Sitosterol (Triple Crown) and androst-1-ene-3,11,17-trione (Sigma) were used as internal standards for quantitative determination by GC (for cholesterol and AD, respectively). Additional standards were 9OHAD, AD and ADD (Koch-Light).
Growth of wild-type and mutant M. smegmatis strains on cholesterol or AD.
NB medium (100 ml in 1 l flasks) was inoculated with M. smegmatis and incubated overnight at 37 °C with shaking at 130 r.p.m. min1. From this culture 20 ml was transferred to 180 ml fresh NB medium in 1 l flasks. At the time of inoculation, cholesterol or AD (0·10·3 g l1) were added to the medium and the cultures were incubated on a shaker (130 r.p.m.) at 37 °C. To determine the dry cell mass at the start of the experiments and at 24 h time intervals, samples (2x5 ml) were withdrawn from the culture, filtered through Synpor filters (pore diameter 0·2 µm) of known weight and the sediment was dried to constant weight.
To determine the progress in cholesterol or AD biotransformation, 2 ml culture samples were taken, mixed with
-sitosterol and androst-1-ene-3,11,17-trione as internal standards (each at 100 µg in 50 µl chloroform), and extracted three times with an equal volume of chloroform. The extracts were dried under vacuum, the residue was dissolved in 0·5 ml acetone and steroids were analysed by chromatography as described previously (Rumijowska et al., 1997
).
To prepare cholesterol or AD, the substrate was dissolved in 5 ml 96 % warm ethanol and an equal volume of sterile distilled water was added. Then the mixture was micronized for 20 min using a water bath/ultrasonic cleaner.
An overnight culture of M. smegmatis (100 ml in 1 l flasks) grown in NB medium was harvested by centrifugation for 20 min at 4000 r.p.m. The cells were resuspended in 10 ml mineral medium and a 2 ml sample was transferred to 198 ml fresh mineral medium in 1 l flasks. Cholesterol or AD was added as sole carbon source. Progress in dry cell mass production and cholesterol or AD biotransformation were monitored. The concentration of the substrate was determined in each experiment.
The enzymic activity of each strain was measured by using GC in at least three independent experiments.
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RESULTS
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The putative ksdD genes in M. smegmatis
The M. tuberculosis genome sequencing project (Cole et al., 1998
) revealed a putative ksdD gene (Rv3537/MT3641) exhibiting about 34 % identity with Arthrobacter simplex and Rhodococcus rhodochrous ksdD products at the amino acid level and an additional ORF (MT0809) with limited homology to a known KsdD (25 % identity with KsdD of A. simplex). Recently the genome sequence of M. smegmatis was annotated. There are as many as six ORFs (MSMEG2871, 2873, 4850, 4855, 5801 and 5898) identified as putative ksdD genes, including those analysed in this paper. The most significant similarity values for each M. smegmatis and M. tuberculosis putative ksdD gene are shown in Table 2
. KsdD is a flavoprotein carrying a conservative N-terminal FAD-binding domain with the consensus sequence GSG(A/G)(A/G)(A/G)X17E (Geize et al., 2000
). Such a motif can be identified in MSMEG5898, MSMEG4850 and MT3641, but not in the other five ORFs analysed (Fig. 2
). Two putative ksdD genes of M. smegmatis, ksdD-1 (MSMEG5898) and ksdD-2 (MSMEG4855), displaying respectively high (78 %) and low (33 %) amino acid sequence identity with the putative ksdD gene of M. tuberculosis (MT3641), were selected for this study. The alignment of putative KsdDs revealed that ksdD-1 (MSMEG5898) is the most probable counterpart of the putative M. tuberculosis ksdD gene (MT3641) and that ksdD-2 (MSMEG4855) shows limited homology to both putative M. tuberculosis ksdD genes MT3641 and MT0809 (33 and 20 %, respectively). Both M. smegmatis KsdDs contain the putative N-terminal FAD-binding motif with one exception, S to T in KsdD2, but we do not know the significance of this variation.

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Fig. 2. N-terminal FAD-binding motif of the putative mycobacterial KsdD. 1, MTB3641; 2, MSMEG5898; 3, MSMEG2871; 4, MSMEG5801; 5, MTB0809; 6, MSMEG4855; 7, MSMEG2873; 8, MSMEG4850. The putative FAD-binding consensus sequence is marked by asterisks.
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Targeted disruption of ksdD-1 results in accumulation of cholesterol degradation intermediates
Our preliminary study revealed that M. smegmatis has the ability to use cholesterol as a source of carbon and energy. Culturing of M. smegmatis in the presence of cholesterol results in fast (about 48 h) complete degradation of this substrate without accumulation of intermediate steroid compounds. The two-step recombination protocol of Parish & Stoker (2000)
was used to obtain the unmarked deletion of the ksdD-1 gene from the M. smegmatis chromosome as described in Methods. The resultant mutant was verified by PCR and Southern hybridization (Fig. 3
). TLC analysis revealed the accumulation of AD when a mutant M. smegmatis strain,
ksdD-1 (DCO1), but not a wild-type M. smegmatis strain, was cultured in the presence of cholesterol (data not shown). To quantify the results obtained, GC analysis, with androsterone and
-sitosterol as the internal standards, was performed. Growth of
ksdD-1 mutant and wild-type M. smegmatis strains in the presence of cholesterol results in fast (48 h) degradation of the steroid substrate. However, the intermediates of cholesterol degradation were detected only in the mutant culture (Fig. 4
). The expected accumulation of AD indicates the inhibition of the cholesterol degradation pathway at the KsdD step. Maximum AD accumulation was observed in a 48-h-old culture of the DCO1 mutant and its presence for the next 192 h indicated that ksdD-1 is essential for degradation of androstendione in M. smegmatis cultured under the conditions used. To confirm that the observed effect was due to unmarked deletion of the ksdD-1 gene, the ksdD gene of M. smegmatis was amplified and cloned in the pJam2 expression vector under the acetamidase promoter and introduced into the DCO1 mutant. The resultant complemented strain was cultured in the presence of cholesterol and acetamide (0·2 %) to induce the expression of the plasmid copy of ksdD-1 and the cholesterol degradation process was monitored by GC. Fast and complete degradation of cholesterol, without accumulation of detectable amounts of steroid degradation intermediates, was observed (data not shown). In the control culture (M. smegmatis
ksdD-1) we found that acetamide per se has no effect on cholesterol degradation and accumulation of AD.
KsdD2 exhibits low but detectable activity in the cholesterol degradation process
M. smegmatis KsdD2 exhibits limited homology to other KsdDs and its FAD-binding motif is not fully conserved. We asked the question whether KsdD2 can participate in the cholesterol degradation process in the wild-type M. smegmatis strain or in the DCO1 mutant. The ksdD-2 gene of M. smegmatis was PCR-amplified and cloned into the pJam2 vector under control of the acetamidase promoter. The resulting construct (pJam2-ksdD-2) was electroporated into the DCO1 mutant to obtain strain DCO1-ksdD-2. Culturing of this strain in the presence of cholesterol results in the degradation of substrate and accumulation of steroid degradation intermediate compounds which were monitored by GC (Fig. 5
). Until the 96 h time point the accumulation of AD was observed, then the amount of AD began to decrease with a simultaneous increase in ADD. This result indicates that KsdD2 exhibits at least a low activity of KsdD after its accumulation in M. smegmatis cells. To test the significance of KsdD2 in M. smegmatis cholesterol degradation, a ksdD-2 gene knock-out in wild-type M. smegmatis and the DCO1 mutant was performed. For unmarked ksdD-2 gene deletion mutagenesis, plasmid pAB46 was constructed and introduced into wild-type M. smegmatis and the DCO1 mutant. The selected ksdD-2 knock-out strains were analysed by PCR and Southern hybridization (Fig. 6
). The obtained mutants, M. smegmatis
ksdD-2 (DCO2) and M. smegmatis
ksdD-1
ksdD-2 (dDCO1,2), were cultured in the presence of cholesterol. The degradation of cholesterol and accumulation of the steroid intermediates were monitored by GC. Both mutants were able to use cholesterol for 48 h as described for the wild-type strain (Fig. 5
). The DCO2 mutant was shown to accumulate a small amount of AD [<1 mg l1 (g dry mass)1] and ADD in the first 2448 h of the biotransformation process. After 4872 h, steroids were not detectable, probably due to KsdD1 activity. The double mutant dDCO1,2 transformed cholesterol to AD, which was stably maintained until 192 h of culture (Fig. 5
). Moreover, ADD was not detectable at any time point, suggesting that KsdD activity was completely inhibited in the dDCO1,2 mutant growing under the given conditions. Furthermore, the pJam2-ksdD-2 construct was introduced into the dDCO1,2 mutant to confirm the activity of KsdD2. The dDCO1,2 mutant carrying the plasmid copy of ksdD-2 gene under a strong, inducible promoter restored KsdD activity manifested by the conversion of AD to ADD which was detectable after 96 h of culture as observed previously for the DCO1-ksdD-2 strain (Fig. 5
).

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Fig. 5. GC analysis of accumulation of AD/9OHAD and ADD produced in cultures of M. smegmatis mutants (M. smegmatis ksdD-1 harbouring plasmid pAB42 with ksdD-2 gene under the control of Pami, DCO1-ksdD-2; M. smegmatis ksdD-2, DCO2; M. smegmatis ksdD-1 ksdD-2, dDCO1,2; M. smegmatis ksdD-1 ksdD-2 with pAB42 plasmid, dDCO1,2-ksdD-2); cultured in rich medium (NB broth) in the presence of cholesterol. The accumulation of AD/9OHAD is marked by filled squares (DCO1-ksdD-2), filled triangles (DCO2), filled circles (dDCO1,2-ksdD-2) and asterisks (dDCO1,2). The accumulation of ADD (if any) is marked by open squares (DCO1-ksdD-2), open triangles (DCO2) and open circles (dDCO1,2-ksdD-2). ADD was not detected in dDCO1,2 mutant culture. The AD/9OHAD ratio was about 1 : 1 in DCO2 and DCO2-ksdD-2 mutants. In the other cases there was as little as 020 % 9OHAD in the AD/9OHAD mixture.
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Fig. 6. Gene replacement of the wild-type ksdD-2 with mutated sequence in M. smegmatis wild-type strain and M. smegmatis DCO1 mutant confirmed by PCR and Southern hybridization. (a) The chromosomal localization of ksdD-2 gene is represented by the grey arrow. The KpnI recognition site is denoted by single letter K. KpnI KpnI distance, ksdD-2 gene size and size of internal deletion in ksdD-2 mutated copy are shown. The brick rectangle represents the deleted part in the mutated copy of ksdD-2. (b) PCR amplification of ksdD-2 gene with MsD2s and MsD2r primers based on plasmid DNA pAB46 (AB46) and chromosomal DNA isolated from wild-type and mutant strains (M. smegmatis mc2 155, mc2; single cross over recombination mutant, SCO; double cross over recombination mutant, mutDCO; double cross over recombination wild-type, wtDCO). M, 1kb ladder (Promega). The ksdD-2 (1641 bp) or ksdD-2 (1030 bp) PCR products are marked by arrows. (c) Southern hybridization of genomic DNA from wild-type M. smegmatis (mc2) and recombinants (SCO, mutDCO, wtDCO of M. smegmatis ksdD-2 and M. smegmatis d ksdD-1, ksdD-2). The DNA was digested with KpnI restriction enzyme, separated in 1 % agarose gel, transferred onto nylon membrane and hybridized with PCR amplified ksdD-2-probe (MsD2s, MsD2r primers and pAB46 DNA as a template). The expected hybridization bands (3607 bp and 2996 bp) are indicated by arrows.
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M. tuberculosis genome also carries two ksdD genes
The genome of M. tuberculosis (TIGR) contains two putative KsdDs, MT3641 and MT0809. We tested if these genes are able to complement the M. smegmatis
ksdD-1
ksdD-2 double mutant. Both genes were PCR-amplified and cloned under control of the Phsp promoter. The resulting constructs were introduced into the mutant cells. GC analysis revealed that overproduction of ksdD-1tb complements the
ksdD-1
ksdD-2 double mutation (Fig. 7
). Initially, cholesterol was biotransformed to AD (48 h) which was further degraded with temporary accumulation of ADD. The pAB43 construct (ksdD-2tb) did not change the ability of the host strain to biotransform cholesterol in comparison to M. smegmatis
ksdD-1
ksdD-2.

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Fig. 7. Cholesterol degradation and AD/9OHAD accumulation by M. smegmatis ksdD-1 ksdD-2 (dDCO1,2), M. smegmatis ksdD-1 ksdD-2 with pAB43 plasmid carrying ksdD-1tb gene under the control of Phsp (dDCO1,2 ksdD-1tb); M. smegmatis ksdD-1 ksdD-2 with pAB49 plasmid carrying ksdD-2tb gene under the control of Phsp (dDCO1,2 ksdD-2tb); cultured in rich medium (NB broth) and monitored by GC. The cholesterol degradation rate is marked by open squares (dDCO1,2), open triangles (dDCO1,2 ksdD-1tb) and open circles (dDCO1,2 ksdD-2tb). The accumulation of AD/9OHAD is marked by filled squares (dDCO1,2), filled triangles (dDCO1,2 ksdD-1tb) and filled circles (dDCO1,2 ksdD-2tb).
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Other KsdD-like enzymes of M. smegmatis are activated when cholesterol or androstendione is the only source of carbon and energy
The above experiments performed in a rich medium would suggest that disruption of ksdD-1 and ksdD-2 in M. smegmatis is sufficient to inhibit completely further degradation of androstendione. In this case the dDCO1,2 mutant would not be able to grow in mineral medium with cholesterol (or AD) as the only source of carbon and energy. However, we found that the wild-type strain as well as the dDCO1,2 mutant can grow on mineral agar plates or in mineral liquid medium supplemented with cholesterol or AD, but not without these sources of carbon. Nevertheless, dDCO1,2 mutant growth was significantly delayed compared to the wild-type strain (data not shown). The GC analysis revealed that the dDCO1,2 strain cultured in mineral medium supplemented with cholesterol accumulated 9OHAD or AD as observed in the rich medium culture. However, the dDCO1,2 mutant growing in mineral medium with AD caused a decrease in the amount of substrate and accumulated ADD starting at the 48 h point. The use of AD by the mutant strain was significantly slower in comparison to the wild-type strain (Fig. 8
). It is very likely that the mineral medium with AD or cholesterol as a sole source of carbon and energy induced the expression of ksdD-like genes (see Table 2
) which are not expressed in rich medium. This expression would allow dDCO1,2 to convert AD to ADD which can be further degraded.
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DISCUSSION
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We identified MSMEG5898 (KsdD-1) as the main KsdD in M. smegmatis. The disruption of ksdD-1 results in the accumulation of AD or 9OHAD in the cholesterol degradation process. However, the M. smegmatis genome contains five other putative ksdD genes. Slight perturbations in cholesterol degradation were also observed due to unmarked deletion of MSMEG4855 (ksdD-2). Moreover, the overexpression of this gene in the M. smegmatis
ksdD-1 mutant complemented the mutant ksdD-1 gene and restored KsdD activity. The double mutant, lacking both ksdD-1 and ksdD-2 genes, accumulated AD in the cholesterol degradation process performed in rich medium, but was able to grow in mineral medium with cholesterol (or AD) as the sole source of carbon and energy. This clearly showed the presence of at least one additional KsdD enzyme responsible for AD dehydrogenation. Two KsdDs were previously described in R. erythropolis and each enzyme alone was able to support the degradation of 9OHAD (Geize et al., 2002
). However, the double disruption of both kstD and kstD2 genes resulted in a metabolic block at the level of 9OHAD. It is interesting that disruption of kstD or kstD2 genes in R. erythropolis resulted in the accumulation of 9OHAD (Geize et al., 2002
). In the case of M. smegmatis the 9OHAD was observed exclusively when cholesterol but not AD was used as a substrate (Wovcha et al., 1979
). This would suggest differences in the steroid degradation pathways in R. erythropolis and M. smegmatis.
Two distinct KsdD activities have also been reported in Mycobacterium fortuitum. Crude extracts of cells induced by AD exhibited
1 dehydrogenation activity to AD and much weaker activity (four times) to 9OHAD. In contrast, cultures induced with 9OH-progesterone were found to show a two-times higher level of
1 dehydrogenation activity to 9OHAD than to AD. However, the particular genes encoding these enzymes remain unknown (Wovcha et al., 1979
). An extra ksdD-like gene (ORF3) was also reported in the A. simplex genome, but its activity was not confirmed (Dziadek et al., 1998
).
In contrast to M. smegmatis, the genome of M. tuberculosis contains only two putative ksdD genes, MT3641 and MT0809 (TIGR). Moreover, the N-terminal FAD-binding motif is not conserved in MT0809. Since the amino acid identity is over 80 %, it is likely that the counterpart of MT3641 in the M. smegmatis genome is MSMEG5898 (ksdD-1). We also found that MT3641 (but not MT0809) was able to complement KsdD activity when overproduced in M. smegmatis dDCO1,2. The genome of M. smegmatis is much bigger in comparison to M. tuberculosis (6·9/4·4 Mb). It is likely that the number of genes has decreased in the course of evolution, since the huge enzymic machinery important for environmental strains could probably be decreased in pathogenic bacteria growing in much more defined conditions. The presence of MT0809 in the M. tuberculosis genome and its low level of homology to known non-mycobacterial ksdD genes would suggest a specific enzyme activity distinct from KsdD1 of M. smegmatis or M. tuberculosis. The most likely counterpart of MT0809 in the M. smegmatis genome is MSMEG5801 (78 % identity at amino acid level) which also lacks the conserved N-terminal FAD-binding sequence. However, further investigations would be necessary to identify the significance of MT0809 and MSMEG5801 for steroid bioconversion.
The significant accumulation of AD by M. smegmatis
ksdD-1 in the biotransformation of cholesterol suggests that the other KsdD-like enzymes (including KsdD2) exhibit low activity or a low expression level in rich medium. The overproduction of KsdD2 in the M. smegmatis
ksdD-1 mutant resulted in the accumulation of AD in the first 72 h of the cholesterol degradation process and subsequent bioconversion of AD to ADD. Our previous investigations showed that the time of maximal activation of Pami in the presence of 0·2 % acetamide is 36 h. Moreover, the activated Pami was able to produce about 250 000 FtsZ molecules per M. smegmatis cell (Dziadek et al., 2002
). On the other hand, the complementation of M. smegmatis
ksdD-1 by ksdD-1, expressed under control of the same promoter (Pami), resulted in fast (48 h) degradation of cholesterol without the accumulation of steroid intermediates as observed in the wild-type strain. The low activity of KsdD2 and potentially of the other KsdD-like enzymes of M. smegmatis could be due to different substrate specificity of these enzymes. It is likely that a particular KsdD-like enzyme uses a different substrate for dehydrogenation and the other substrates are less preferred. We observed the accumulation of an unrecognized product (probably C2224 acids) in the cholesterol degradation process carried out by strains lacking ksdD-2 which did not accumulate in M. smegmatis
ksdD-1. However, to understand the significance of all putative KsdDs in steroid biotransformation and their substrate specificity, further investigations, including construction of mutants, protein purification and analysis, would be required.
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ACKNOWLEDGEMENTS
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The work was supported by grants from the State Committee for Scientific Research (KBN, contracts nos. 3P05A14024 and 3P04B00224). We thank Dr T. Parish for the pJam2 expression vector and p2NIL/pGOAL17 recombination system.
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Received 8 February 2005;
revised 24 March 2005;
accepted 24 March 2005.
Copyright © 2005 Society for General Microbiology.