Bacterial strains and culture conditions

The bacterial strains and plasmids used in this study are described in Table S1. All cloning experiments were performed in Escherichia coli DH10B, cultivated in Luria-Bertani (LB) broth at 37°C or on LB agar containing 50 µg kanamycin, for 16 hours at 37°C. Mycobacterial strains were grown in Middlebrook 7H9 medium (Difco) supplemented with albumin (6.25% (w/v)), dextrose (2.5% (w/v)), sodium chloride (1.1% (w/v)), catalase (5×10⁻⁴% (w/v)) and 0.05% (v/v) Tween−80 at 37°C for Mycobacterium smegmatis and 30°C for M. marinum and M. ulcerans. Mycobacteria were also cultured on 7H10 agar supplemented with OADC (Difco). Recombinant mycobacteria were cultivated with kanamycin at a final concentration of 25 µg ml⁻¹.

DNA methods

Standard methods were used for cloning, PCR and DNA sequencing. The oligonucleotides used in this study for PCR, RT-PCR and DNA sequencing are listed in Table S2. Genomic DNA was extracted from mycobacteria as described [23]. The broad host range, promoterless, GFP (gfpmut3) vector pSM20, that replicates in E. coli, Corynebacterium sp. and Mycobacterium sp, was used for all promoter cloning experiments [32]. PCR products derived from the upstream regions were modified using oligonucleotides described in Table S2 and ligated into the unique restriction enzyme sites immediately upstream of the gfp gene in pSM20 (Figure 1). Constructs were confirmed to be correct by DNA sequencing and then transformed into M. smegmatis mc²155 as described [33]. Electrocompetent M. marinum and M. ulcerans were prepared as described [34] and these cells were transformed with 10 µg of DNA from plasmid pJKD2893 (Table S1). The constructs were confirmed to be correct in mycobacteria by Southern hybridization and back transformation to E. coli. Acetone soluble lipids were extracted from recombinant M. ulcerans and analysed by LC-MS for the presence of mycolactones as previously described [35].

Measurement of green fluorescence protein (GFP) expression

GFP expression in pSM20 and derivatives (Table S1) was measured using a FLUOstar OPTIMA plate scanner (BMG Lab Technologies). M. smegmatis strains were grown to an OD of 1.0 using a WPA CO8000 cell density meter (Isogen Life Science). For each strain, 30 µl of starter culture was added to each of 16 wells of a 96-well flat-bottomed clear plate containing 150 µl of fresh 7H9 medium. Plates were incubated at 37°C for 30 mins. Each well was scanned using an excitation filter of 485 nm and an emission filter of 520 nm. Fluorescence readings were taken every 10 minutes and the average of 20 flashes per well was taken to be the measure of fluorescence. Prior to each reading, the plates were shaken for 5 minutes in an orbital motion. Replicates were averaged for each experiment and the average value for the vector-only control was taken as background and subtracted from the average at each time point.

Preparation of total RNA

Total RNA was prepared from E. coli using the RNeasy mini kit as described and per the manufacturer's instructions (Qiagen) [36]. For M. ulcerans, a 0.5 volume of RNAlater (Qiagen) was added to 100 ml of late log-phase culture and allowed to stand at room temperature for 10 minutes prior to centrifugation at 4,600 g, for 10 minutes. The resultant cell pellet was washed in 1 ml of 0.5% (v/v) Tween-80 per 50 mg of cells (wet weight), resuspended in 800 µl of RNA lysis buffer (0.12 M sodium acetate (pH 4.0), 9.6% (v/v) liquid Pyroneg (Diversey), pH 4.0) and then added to 250 µg of glass beads (Sigma Aldrich), with 600 µl of acidified phenol:chloroform (pH 4.0) (Sigma Aldrich). Cells were disrupted with a FastPrep tissue homogenizer (Savant Instruments) for 45 seconds, at speed 6 and chilled on ice for 5 minutes. The aqueous phase was then re-extracted with chloroform:isoamylalcohol (24:1) and precipitated with isopropanol, and 3 M sodium acetate (pH 4.6). Two 70% (v/v) ethanol washes were performed and the pellet was dried briefly under vacuum and resuspended in 100 µl of DEPC water. RNA in this preparation was then further purified using an RNeasy extraction kit, including an on-column DNase treatment, following the manufacturers recommendations (Qiagen). For RNA extraction from M. smegmatis and M. marinum the following modifications to the above method were used. The cell pellet was first resuspended in 2 ml of lysis solution (20 mM potassium acetate (pH 4.8), 1 mM EDTA, 0.5% (v/v) SDS, 100 µg proteinase K ml⁻¹). One millilitre was added to 250 µg of glass beads with 700 µl acidified phenol:chloroform pH 4.0. Cells were disrupted by three cycles in a FastPrep instrument at speed 5, for 30 seconds, and then centrifuged at 17,900 g for 10 minutes. The aqueous phase was recovered and extracted once with 500 µl phenol:chloroform (pH 4.0) followed by a chloroform only extraction. Nucleic acids were precipitated as above and RNA extraction proceeded as for M. ulcerans using the RNeasy extraction kit.

Primer extension

The primer extension protocol used was modified from Lloyd et al., [37]. Two reverse transcription reactions were performed. To the RNA-primer mix, 6 µl of 5x first strand buffer (Invitrogen), 15 mM DTT (Invitrogen), 1 mM dNTPs (Promega), 1 U RNasin (Promega) and 100 U of Superscript II RNase H^- reverse transcriptase (Invitrogen) were added. After one hour at 42°C, 2 µl of 5x first strand buffer, 1.5 mM dNTPs, 1 U RNasin, 15 mM DTT and 100 U of Superscript II was added and incubated for a further hour at 42°C. Ten nanograms of RNaseA (Sigma) was then added and allowed to incubate at 37°C for 30 minutes. The resultant cDNA was precipitated and washed once with 70% (v/v) ethanol, dried and stored at −20°C until analysis. Capillary electrophoresis was performed on an Applied Biosystems 3730 DNA analyzer using Liz™ 500 size standards to generate a standard curve (Applied Biosystems). Genemapper® version 3.7 (Applied Biosystems) was used to analyze the sample files with automated allele calling verified by manual inspection. The sized cDNA fragments were then mapped to their respective first strand synthesis primer binding sites to identify the putative transcription start site.

Bioinformatic analysis

From the alignment of each of the SigA, C, D, E, F, H & L promoters [38], nucleotide frequency counts were derived and used to construct a library of 110 position specific scoring matrices (PSSMs) for each sigma factor (PSSMs available upon request). This allowed the gap between the -35 and -10 signals to vary between 14 and 23 residues, and the gap between the -10 signal and the TSP to vary between 3 and 13 residues. PoSSuM software [39] was used to scan the pMUM001 genome for high scoring hits to these PSSM libraries [40], using a background model consistent with the G+C biased nucleotide distribution of pMUM001. A p-value significance cutoff of 0.0001 was used.

Site-directed mutagenesis

Splice overlap extension PCR [41] was used to alter the sequence of putative promoter motifs with oligonucleotides 1075-F and 1074-R for mlsA1/mlsB, 1667-F and 1668-R for mup045, and 1669-F and 1670-R for mup053 (Table S2). Each PCR reaction consisted of 20 cycles of 94°C for 1 minute, 50°C for 1 minute and 72°C for 3 minutes then 94°C for 1 minute, 72°C for 10 minutes and held at 4°C. Two overlapping PCR products were obtained and 2 µl (∼50 ng DNA) of each were used in a subsequent reaction using the outermost primers for each product to yield a complete fragment incorporating both products. Each product was then ligated into pSM20 as described above. Mutations were confirmed by DNA sequencing.

Mouse-tail infections

Ten, six-week-old female BALB/c mice (Charles River France, http://www.criver.com/) were injected subcutaneously into the tail with 30 µl of a suspension containing 5×10⁴ bacteria. To favour the growth of the GFP-expressing bacilli, animals received 0.1 ml of a solution containing 80 mg/ml of kanamycin (1% w/v), administered by oral gavage every day. The mice were killed and their tails were collected fifty days after inoculation.

Ethics statement

Mice were maintained in the animal house facility of the Centre Hospitalier Universitaire, Angers, France (Animal Ethics Committee, Centre Hospitalier Universitaire, Agreement A 49 007 002), adhering to the institution's guidelines for animal husbandry.

Detection of cultivable bacilli and histology

The tissue specimens from mice were minced with disposable scalpels in a Petri dish and ground with a Potter–Elvehjem homogeniser, size 22, (Kimble/Kontes, Vineland, NJ), in 0.15 M NaCl to obtain a tenfold dilution. The suspension was decontaminated to remove other bacteria using an equal volume of N-acetyl-L-cysteine sodium hydroxide (2%) [42] and inoculated on 7H10 agar supplemented with OADC (Difco), containing 25 µg/ml of kanamycin. For histological examination, tissues were fixed in 4% paraformaldehyde in phosphate buffer (pH 7.4). Decalcification of the tissue was performed for 7 days in 0.1 M of EDTA solution in PBS. Samples were frozen in isopentane cooled to −140°C in liquid nitrogen and stored at −80°C for subsequent histochemical analysis. Eight-micron thick transverse sections were cut at −30°C on a cryostat (Jung-Reichert Cryocut 1800, Cambridge Instruments, Germany) and kept at −80°C until histochemical processing, which was done within 1 week of sectioning. For detection of GFP-expressing bacilli, tissues were counterstained with DAPI, with endogenous phosphatase activity first detected using alkaline phosphatase substrate kit I (Vector Laboratories). The preparation was then mounted in Vectashield mounting medium containing DAPI (Vector Laboratories) and the samples were visualized using fluorescence microscopy (Leica DM5000B). Hematoxylin phloxine saffron and Ziehl Nielsen staining were performed according to standard procedures.

Mosquito microcosm M. ulcerans-GFP feeding experiments

Mosquito larvae (Aedes camptorhynchus) between first and second instar were distributed into 4×50 ml plastic tubes (10 larvae per tube), containing 20 ml of sterile tap water. To three groups of four tubes were added 1.5 ml of an aqueous slurry of possum faecal material containing either 5×10⁶ colony forming units (cfu) M. ulcerans-GFP, 5×10⁶ cfu M. marinum-GFP, or possum faecal material alone. The larvae were left to feed on the material for one week at 24°C. At the end of one week and also at the end of every subsequent week up to week five, all larvae were transferred to new tubes containing 20 ml of sterilized tap water. The original tubes spiked with possum faecal material were kept at room temperature and at the commencement of each week 500 µl of water from each of these tubes was tested by IS2404 and ppk qPCR to estimate the residual quantity in the water of M. ulcerans and M. marinum respectively [43]. Results were reported as cfu by reference to standard curves for each PCR and bacterial species, correlating qPCR Ct values with cfu [43]. From weeks 2–5 the larvae were sustained with small quantities of fish food added to each tube. A larva was taken from each tube as it progressed through each instar and tested by IS2404 PCR for the presence of M. ulcerans as described [43]. A selection of 4^th instar larvae were also fixed overnight in 10% formaldehyde in PBS (v/v) then mounted in cedarwood oil (Matheson, Coleman and Bell) on a glass slide for examination by fluorescence microscopy with an Olympus BX51 microscope (Olympus, Tokyo, Japan) with the following filter sets: DAPI (Blue) ex: 360–70 nm, em: 420–60 nm, FITC (Green) ex: 450–80 nm, em: 535 nm, TRITC (red) ex: 535 nm, em: 635 nm. Images were acquired using an Olympus DP-70 digital camera and merged using DP controller software (version 1.1.1.71) or Adobe Photoshop (version 8) These experiments were terminated before the insects progressed to pupal and adult developmental stages.

Identification of promoter regions in mycolactone-associated genes using a GFP-reporter

By cloning DNA fragments ranging from 229 bp–1646 bp located immediately upstream of mlsA1/mlsB (these genes have a duplicated start and upstream sequence so one cloned fragment was sufficient to analyse both genes), mlsA2, mup038, mup045 and mup053 in the promoterless GFP E. coli/Mycobacterium reporter vector pSM20 (Table S1, Figure 1) we were able to discover regions containing promoter activities. The resulting plasmids were used to transform E. coli, M. smegmatis and, for the mlsA1/mlsB construct, M. marinum and M. ulcerans were also transformed. Bacteria were cultured in 96-well plates for 2 hours at 37°C and expression of GFP for each strain was assessed by continuous fluorescence measurements. E. coli expressing GFP from the strong, constitutive promoter srp (pSM22) [32] and M. smegmatis expressing GFP from the sigA promoter from Mycobacterium bovis BCG (pJKD3042) [44] were used as positive controls for each genus. Results were expressed as fold changes in fluorescence above the levels detected in bacteria containing the empty vector pSM20. The results for mlsA1 and mlsB are summarized in Figure 2 and show that strains containing the construct pJKD2893 with the region 1646 bp upstream of mlsA1/mlsB, led to detectable GFP expression in E. coli, and high levels of GFP expression in M. smegmatis and M. marinum (Figure 2A). A single copy version of pJKD2893 was also created where a DNA fragment spanning the 1646 bp mls upstream region and gfp gene from pJKD2893 was subcloned into the mycobacterial integrating shuttle vector, pJKD8003 resulting in pJKD3111. M. marinum transformed with pJKD3111 expressed GFP 40-fold less than the same strain containing pJKD2893 (Figure 2A).

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Figure 2. Summary of fluorescence data demonstrating the difference in promoter activity among strains containing GFP reporter constructs.

Shown are plasmid constructs with upstream regions from M. ulcerans mlsA1/mlsB (A) & (B). Also shown are the sigA promoter from M. bovis BCG (construct pJKD3042) (B) and the srp promoter from E. coli (construct pSM22) (B). Point mutations in putative promoter regions in the putative -10 motifs of promoter regions for mls sequences are marked by ‘X’. All values are expressed as fold changes above the strain containing the empty vector pSM20. Strains are identifiable by a two-letter prefix to the strain number EC - E. coli, MS - M. smegmatis, MM - M. marinum and MU - M. ulcerans. ‘*’ indicates this fluorescence is more than 100-fold higher than vector alone.

https://doi.org/10.1371/journal.pntd.0000553.g002

To further localize the region conferring promoter activity within the 1646 bp upstream of mlsA1/mlsB, four overlapping sub-clones of this region were prepared by PCR, cloned into pSM20 and used to transform E. coli and M. smegmatis. Comparison of GFP expression in these constructs in another time course experiment, comparing fluorescence with the full-length 1646 bp fragment and controls, clearly showed that promoter activity was restricted to a 413 bp fragment located between nucleotide positions 35996-36409 for mlsA1 and 100821-101234 for mlsB in pMUM001 (Figure 2B).

The region 1440 bp upstream of mup045 and 1466 bp upstream of mup053 also led to significant GFP expression in M. smegmatis, 8–15 fold above background, but these regions showed little transcriptional activity in E. coli (Figure S1). No fluorescence was observed in either E. coli or M. smegmatis for strains containing the 229 bp region upstream of mup038 (pJKD3269) or the 1096 bp region upstream of mlsA2 (pJKD3041) (data not shown). These experiments demonstrate that the regions upstream from mlsA1/mlsB, mup045 and mup053 all harbour at least one strong promoter.

Identification of transcriptional start points (TSPs) for mlsA1/mlsB, mup045, and mup053

To identify TSPs upstream of each gene primer extension (PE) analysis was performed using RNA extracted from M. ulcerans Agy99. For mlsA1/mlsB, RNA was also extracted from M. marinum harbouring the GFP expression construct pJKD2893. One or more 5′ 6-FAM-labeled antisense oligonucleotides were used to prime cDNA synthesis to determine the TSP for mlsA1/mlsB, mup045, and mup053 (Table S2). Single, distinct PE products were identified for all three regions using multiple RNA preparations (Figure S2, Figure S3). Size fragment analysis of the PE products suggested single TSPs at 533 bp (T533) upstream of the mlsA1/mlsB translational start (Figure S2), 207 bp upstream of mup045 (T207), and 68 bp upstream of mup053 (T068) (Figure S3). Primer extension analysis of mup038 and mlsA2 was not attempted due to the lack of promoter activity observed with the wild type sequences in the GFP reporter assays.

Localization of putative promoter sequences by in silico analysis

Several studies of promoters in mycobacteria facilitated the construction of position-specific scoring matrices (PSSMs) to perform in silico searches for potential regulatory regions in DNA sequences [38]. We used sigma factor-specific libraries of PSSMs to scan the regions upstream of the three TSPs identified by our PE analysis. High-probability SigA-like promoter motifs were predicted in the regions upstream of mlsA1/mlsB and mup045 and a SigD-like motif was predicted upstream of mup053 (Table 1).

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Table 1. Comparison of mycolactone promoter sequences with mycobacterial consensus sequences.

https://doi.org/10.1371/journal.pntd.0000553.t001

Confirmation of putative promoter elements by site-directed mutagenesis

To confirm the in silico promoter predictions, the GFP expression constructs spanning the putative -10 sequences from mlsA1/mlsB (pJKD2893), mup045 (pJKD3040) and mup053 (pJKD3039) were mutated by PCR (Table 1). GFP production by E. coli and M. smegmatis harbouring these constructs was assayed as before by continuous fluorescence measurements over 2 hours at 37°C. Fluorescence production was compared with the same strains containing the wild-type putative promoter sequences. Mutation of the proposed −10 boxes for both the mlsA1/mlsB and mup045 reduced fluorescence in M. smegmatis to less than 4% of the wild-type sequences, strongly suggesting these sequences are functional −10 motifs, required for proper binding of the sigma factor and RNA polymerase to initiate transcription (Figure 2B). Mutation of the proposed −10 box from mup053 had no impact on GFP expression.

Construction and analysis of M. ulcerans expressing GFP under the control of the mlsA1/mlsB promoter

The strength of the mls promoter led us to develop a GFP-producing strain of M. ulcerans that might be useful in studies of pathogenesis or transmission. We transformed M. ulcerans JKD8049 with plasmid pJKD2893, resulting in highly green fluorescent M. ulcerans (JKD8083 or M. ulcerans-GFP), with fluorescence expression more than 100 fold above empty vector (Figure 2A). To ensure that GFP expression did not stop mycolactone production we performed cell LC-MS analysis of acetone-soluble lipids from cultures of JKD8083 and confirmed the presence of mycolactone A/B and C (Figure S4).

M. ulcerans-GFP retains virulence in vivo

Mouse-tail infection is a well-established animal model for studying M. ulcerans. Forty days after subcutaneous inoculation of 10⁵ M. ulcerans-GFP oedema was observed and on the 50^th day the lesion became ulcerated and the mice were killed. Histological study of the ulcerated region showed an area of necrosis consistent with wild type M. ulcerans infection (Figure 3A, Figure 3B). Granulomatous inflammation was not observed. Acid-fast bacilli were localized in clumps in necrotic areas (Figure 3C) and expressed green fluorescent protein (Figure 3D). The viability of these bacteria was demonstrated by re-isolating them in bacterial culture media. These results demonstrate that M. ulcerans-GFP is virulent in the mouse model and provokes lesions typical of M. ulcerans infection.

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Figure 3. Histological study of serial mouse tail sections following mouse-tail infection with M. ulcerans-GFP.

(A) Fifty days after subcutaneous inoculation in the tail of 10⁵ bacilli showing the beginning of ulceration. (B) Hematoxylin phloxine saffron staining on tissue section reveals massive necrosis. (C) Ziehl-Nieelsen staining showing many extracellular individual and clustered bacilli (arrowheads) associated with necrosis, and (D) bacilli expressing GFP. Scale bars: 0.8 cm (A), 100 µm (B, C, and D) and 40 µm (C and D insets).

https://doi.org/10.1371/journal.pntd.0000553.g003

M. ulcerans-GFP accumulates within mosquito larvae

Adult mosquitoes in some Buruli ulcer endemic regions of Australia have tested PCR positive for M. ulcerans and epidemiological evidence suggests a role for biting insects in the disease ecology of M. ulcerans [45],[46]. These data and the presence of M. ulcerans in possum faecal material from the same endemic regions has led to the hypothesis that larval stages of mosquitoes may and probably do ingest M. ulcerans as well as other bacteria via filter feeding activity on decomposing, faecally contaminated environments [47]. We mimicked this environment by establishing simple aquatic microcosms, seeded with 1 or 2 instar Aedes camptorhynchus larvae that were then transiently fed with possum faecal material, spiked with either M. ulcerans-GFP or M. marinum-GFP (Figure 4A). M. ulcerans and M. marinum were initially liberated into the water from the food source but neither bacterial species were detectable in water by week 4 (Figure 4B). Analysis of 4^th instar larvae at week 4 by fluorescence microscopy revealed an accumulation of M. ulcerans primarily within the larval midgut and around the mouthpart (Figure 4C). Fourth instar larvae assayed by PCR for M. ulcerans had a mean bacterial load of 27,300±15,200 cfu (n = 4). The same pattern of accumulation within the insect was not seen with M. marinum-GFP with very few fluorescent bacteria observed in association with larvae (Figure 4C). Neither M. ulcerans or M. marinum were detected in the microcosms containing mosquito larvae only (Figure 4C). These data show that mosquito larvae in contaminated aquatic environments were able to ingest and maintain M. ulcerans within regions of the digestive tract over a significant time period.

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Figure 4. Concentration of M. ulcerans-GFP within 4^th instar mosquito larvae.

(A) Epifluorescence microscopy (x100 objective) demonstrating that the majority of total fluorescent bacteria (DAPI-staining, blue filter) are also GFP-expressing M. ulcerans (JKD8083) and M. marinum (JKD8062) (green filter). (B) Reduction of M. marinum and M. ulcerans within the water of the microcosms over the 4-week duration of the experiment as measured by qPCR. Results are the means and standard deviations of four biological repeats. (C) Bright field, red fluorescence, green fluorescence and composite images showing the accumulation of M. ulcerans around the mouth and mid-gut of a 4^th instar Aedes camptorhynchus larva. Scale bar indicates 0.5 mm. Inset images are ×400 magnification. No specific green fluorescence was observed in larvae infected with M. marinum or uninfected controls. Red fluorescence images were included to show that green fluorescence was due to GFP expression and not autofluorescence.

https://doi.org/10.1371/journal.pntd.0000553.g004