Unité des Cyanobactéries (CNRS URA 2172), Département de Biochimie et Génétique Moléculaire, Institut Pasteur, 28 Rue du Dr Roux, 75724 Paris Cedex 15, France1
Station Biologique de Roscoff (CNRS UPR 9042), BP 74, 29682 Roscoff Cedex, France2
Author for correspondence: Isabelle Iteman. Tel: +33 1 4568 8416. Fax: +33 1 40613042. e-mail: iiteman{at}pasteur.fr
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ABSTRACT |
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Keywords: Prochlorococcus marinus subsp. pastoris PCC 9511T, cyanobacteria, group-specific ITS primers, oceanic, coastal marine and freshwater Synechococcus, secondary structure of the rrn operon
Abbreviations: DV, divinyl; HL, high-light-adapted clade; LL, low-light-adapted clade; ITS, Internal Transcribed Spacer; OMF, oceanic, marine and freshwater; RFLP, restriction fragment length polymorphism
The GenBank accession numbers for the ITS amplicon sequences reported in this paper are AF387607 (PCC 9511T), AF387610 (PCC 6307), AF387608 (PCC 7001) and AF387609 (PCC 7941).
a Present address: Unité de Recherche en Génomique Végétale (INRA/CNRS), Genoscope, Centre National de Séquençage, 2, Rue Gaston Crémieux, 91057 Evry Cedex, France.
b Present address: Carl von Ossietzky University, Geomicrobiology, PO Box 2503, 26111 Oldenburg, Germany.
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INTRODUCTION |
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Based on their preferential habitats, surface waters or deep layers receiving high or low irradiance, respectively, DV-chlorophyll b/a ratios and phylogenetic position deduced from 16S rRNA gene analyses, three subgroups have been recognized among isolates and environmental samples of Prochlorococcus (Morel et al., 1993 ; Partensky et al., 1993
; Moore et al., 1995
, 1998
; Palenik, 1994
; Urbach et al., 1998
; West & Scanlan, 1999
; West et al., 2001
; see also Partensky et al., 1999
). Two of these (HLI and HLII) are group members of the high-light-adapted clades (HL) that proliferate in surface layers of the oceans and have a very low DV-chlorophyll b/a ratio. The third, loosely defined as the low-light-adapted clade (LL), is composed of genetically more diverse ecotypes that exhibit higher DV-chlorophyll b/a ratios and occur preferentially at depths of more than 100 m. However, the vertical positioning is influenced by the degree of stratification of the water columns, more extensive mixing leading to the co-existence of both HL and LL ecotypes at the same depth (Moore et al., 1998
; Ferris & Palenik, 1998
). In addition, the relative abundance and depth distribution of members of the HLI and HLII subclades (West & Scanlan, 1999
) may differ strikingly, depending on the geographical region (West et al., 2001
).
The axenic Prochlorococcus marinus subsp. pastoris strain PCC 9511T has a low mean DNA base composition (32 mol% G+C) and a small genome (2 Mbp) (Rippka et al., 2000 ). However, as inferred from 16S rDNA sequence analysis, the closest phylogenetic relatives of Prochlorococcus isolates or environmental clones (Urbach et al., 1998
; West & Scanlan, 1999
; West et al., 2001
) are some unicellular cyanobacteria of the genetically diverse Synechococcus group (Waterbury & Rippka, 1989
; Turner, 1997
; Honda et al., 1999
; Herdman et al., 2001
). These are all of relatively small diameter (0·81 µm), span a mean DNA base composition in the range of 5570 mol% G+C (Herdman et al., 1979b
, 2001
; Waterbury et al., 1986
; Waterbury & Rippka, 1989
) and (where known) have a genome size of about 4 Mbp (Herdman et al., 1979a
), though that of the oceanic Synechococcus WH8102 is only 2·4 Mbp as shown by the genome sequencing project. Synechococcus strains that cluster most tightly with members of Prochlorococcus, and were thus assigned to the marine picophytoplankton clade (Urbach et al., 1998
), have all been isolated from the open ocean (Waterbury et al., 1986
; Waterbury & Rippka, 1989
) where they often co-exist with Prochlorococcus populations (Chisholm et al., 1988
; Li & Wood, 1988
; Olson et al., 1990
; Shimada et al., 1996
; Partensky et al., 1999
). In contrast, Synechococcus strains that are positioned at the root of the former clade (Urbach et al., 1998
; West & Scanlan, 1999
; Rippka et al., 2000
; West et al., 2001
) are of freshwater origin (Kane et al., 1997
; Postius & Ernst, 1999
), or were isolated from a coastal marine environment (Rippka et al., 2000
). To distinguish the ensemble of these related Synechococcus strains (or environmental clones) from other members of the Synechococcus group, that in 16S rDNA trees are more remote and dispersed in several distinct phylogenetic lineages (Turner, 1997
; Honda et al., 1999
; Herdman et al., 2001
; Robertson et al., 2001
), we shall here refer to them collectively as members of the oceanic, marine and freshwater (OMF)-Synechococcus clade.
For a variety of reasons, precise identification of cyanobacteria by classical bacteriological criteria is difficult (Rippka et al., 1979 ; Castenholz & Waterbury, 1989
), but a number of different PCR-based strategies for the genetic characterization of strains, or environmental samples, are now available. Identification of Prochlorococcus genotypes has been achieved by different molecular approaches (Palenik, 1994
; Ferris & Palenik, 1998
; Scanlan et al., 1996
; Urbach et al., 1998
; West et al., 1999
, 2001
), including single-cell hybridization with labelled probes and detection of the fluorescent signals by light microscopy or flow cytometry (West et al., 2001
; Worden et al., 2000
). However, some of these methods are labour-intensive or are based on relatively conserved RNA polymerase or 16S rRNA gene sequences and thus may not provide sufficient resolution to distinguish between the different Prochlorococcus genotypes with precision. Furthermore, even discrimination of some members of Prochlorococcus from representatives of the OMF-Synechococcus clade may be difficult (West et al., 2001
). Thus, more specific tools for the distinction within and between these two groups of organisms that often share the same ecological niche (Chisholm et al., 1988
; Olson et al., 1990
; Campbell & Vaulot, 1993
; Partensky et al., 1999
) are still desirable.
In a survey of about 320 axenic cyanobacterial strains of the Pasteur Culture Collection of Cyanobacteria (PCC; Institut Pasteur, Paris, France), it was observed that the different sizes of the Internal Transcribed Spacer (ITS) obtained by PCR amplification correlated well (I. Iteman, unpublished results) with particular strain clusters in genetically diverse genera such as Synechococcus or Synechocystis (Waterbury & Rippka, 1989 ; Rippka & Herdman, 1992
; Herdman et al., 2001
). Knowing that the ITS is less conserved than the 16S rRNA gene in cyanobacteria (Wilmotte, 1994
; Neilan et al., 1997
; Otsuka et al., 1999
; Iteman et al., 2000
), we have examined the value of this domain for the genotyping of eight isolates of Prochlorococcus (one axenic, seven non-axenic) by PCR amplification, sequencing and/or RFLP of the ITS regions. For comparison, four Synechococcus strains of the OMF-Synechococcus clade (three axenic, one non-axenic) were also included in this study, one of which (PCC 6307) has previously been proposed as the type strain of Cyanobium gracile gen. nov., sp. nov. Rippka & Cohen-Bazire 1983 (Komárek et al., 1999
; Herdman et al., 2001
). However, since the new genus Cyanobium has not yet been validated under the Bacteriological Code of Nomenclature and may in the future also be applicable to some of the other representatives of the OMF-Synechococcus clade, this nomenclatural change has been avoided here.
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METHODS |
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Cultivation of strains.
All cultures, except strains PCC 6307 and PCC 7001, were grown at 1820 °C in liquid medium PCR-Tu2 (Rippka et al., 2000 ). Strain PCC 6307 was grown at 23 °C in medium BG11 (Rippka et al., 1979
). Strain PCC 7001 was cultivated in a mixture (1:1) of media BG11 and ASNIII (Rippka et al., 1979
). For all strains, white light was supplied by fluorescent tubes providing during a light/dark cycle of 14/10 h a photosynthetic photon flux density (PPFD) of about 20 µm photons m-2 s-1 (measured with a LICOR LI-185B quantum/radiometer/photometer equipped with a LI-190SB quantum sensor). The neon tubes were Duro-Lite (USA) for all strains, except PCC 6307 and PCC 7001, for which illumination was with Universal White neon tubes. The strain of Microcystis aeruginosa, PCC 7941, used in one control experiment, was grown in medium BG11o (Rippka et al., 1979
) supplemented with NaNO3 (2 mM) and NaHCO3 (10 mM) under the light and temperature regimes described for strains PCC 6307 and PCC 7001. Several bacterial contaminants that also served for control PCR reactions were isolated from Prochlorococcus strains MED4 and SS120 on plates of medium PCR-Tu2 supplemented with glucose (0·2%, w/v), Casamino acids (0·002%, w/v) and Luria Broth (5%, v/v) (Sambrook et al., 1989
) and solidified with washed agar (0·8%, w/v) (Rippka et al., 2000
). Incubation was at 20 °C in the dark. The purity of the axenic Prochlorococcus and Synechococcus strains was routinely checked in the appropriate growth medium with the same supplements as described for the isolation of the bacterial contaminants, but solidified with Difco Bacto agar (1%, w/v).
PCR amplification of the ITS region.
Amplification of the ITS regions of Prochlorococcus and Synechococcus strains was performed on cells (12 ml; OD750 about 0·1 for Prochlorococcus and 0·51·0 for Synechococcus) harvested by centrifugation (15 min at 20 °C and 20000 g), washed twice in 150 mM NaCl and resuspended in 50200 µl sterile H2O or TE buffer (10 mM Tris, pH 8·0, 0·1 mM EDTA). Aliquots of the cell suspensions (110 µl) were either used directly for the PCR reactions or after lysis by five alternating cycles of freezing in liquid nitrogen and thawing at 50 °C. The respective standard forward and reverse primers for amplification were 322 (5'-TGTACACACCGCCCGTC-3') and 340 (5'-CTCTGTGTGCCTAGGTATCC-3'), previously employed for cyanobacteria (Wilmotte et al., 1993 ; Iteman et al., 1999
, 2000
). Primer 322 initiates amplification at a region near the end of the 16S rDNA on the RNA-like strand (positions 13381354 in Synechocystis PCC 6803; Escherichia coli numbering 13911407); primer 340 is complementary to a region on the opposite strand at the beginning of the 23S rDNA (positions 2645 in both Synechocystis PCC 6803 and E. coli). For the numbering of the E. coli rrn sequences, see Brosius et al. (1981)
. Alternatively, forward primer 600, designed in this study (5'-CACCTCCTAACAGGGAGACA-3') and corresponding to the last 10 nt of the 16S rDNA (E. coli numbering 15331542) and the first 10 nt of the ITS on the RNA-like strand in the rrn operon of Prochlorococcus PCC 9511, was used in combination with reverse primer 340. The higher specificity of the latter set of primers for the Prochlorococcus and Synechococcus strains was tested by attempting ITS amplification on a cell suspension (1 µl, OD750 about 0·5) of the cyanobacterium Microcystis aeruginosa PCC 7941 and lysates (10 µl) of several bacterial contaminants prepared by alternating cycles of freezing in liquid nitrogen and thawing as described above. PCR amplifications with primers 322 and 340 served as positive controls.
The PCR mixture contained 10 µl Taq commercial buffer (10x) supplemented with MgCl2 to a final concentration of 2 mM, 110 µl cells or lysates as templates, 150 µM each dNTP, 500 ng each primer and 2·5 U Taq polymerase (Promega). The total reaction volume was 50 or 100 µl. Incubation of the reactions was initially performed in a Perkin-Elmer Cetus Gene Amp 9700 Thermal Cycler using the following programme. After an initial cycle consisting of 5 min at 95 °C, 1 min at 55 °C and 30 s at 72 °C, 30 cycles of amplification were started (1 min at 95 °C, 1 min at 55 °C and 1 min at 72 °C). The reaction was terminated by a cycle of 5 min at 72 °C. For later PCR reactions in a Stratagene Robocycler Gradient 40, the programme was modified: 1 cycle consisting of 5 min at 94 °C, 1 min at 55 °C and 30 s at 72 °C; 30 cycles of 30 s at 94 °C, 30 s at 55 °C and 30 s at 72 °C; the final cycle was 1 min at 95 °C, 1 min at 55 °C and 5 min at 72 °C. Storage of the reactions in both programmes was at 4 °C. A negative control without template was included in some experiments. The PCR products were analysed by electrophoresis on 1·5% (w/v) agarose gels (Litex LSL 4000, FMC BioProducts Europe) in 1x TBE (Tris-borate-EDTA) buffer (Sambrook et al., 1989 ), stained with ethidium bromide (0·5 µg ml-1) and photographed under UV light. The length of the DNA fragments was estimated by comparison with a 100 bp DNA ladder (Amersham Pharmacia Biotech).
Cloning and sequencing of the ITS region.
The PCR products of Prochlorococcus PCC 9511T, Synechococcus strains PCC 6307 and PCC 7001, and Microcystis aeruginosa PCC 7941, obtained with primers 322 and 340, were sequenced after cloning or directly on the PCR products as described by Iteman et al. (2000) .
Alignment and analyses of the ITS sequences.
Alignment of the ITS sequences of Prochlorococcus PCC 9511T and Synechococcus PCC 6307 and PCC 7001, together with those of Prochlorococcus MED4 and MIT9313, available from the genome sequencing projects, were made manually using Genedoc v. 2.5 (http://www.psc.edu/biomed/genedoc/) and by reference to the cyanobacterial ITS alignment and secondary structure models of the rRNA transcripts proposed by Iteman et al. (2000) .
Analyses of the 16S rDNAITS overlapping regions.
The sequences of the 16S rDNAITS overlapping regions of Prochlorococcus MED4 and MIT9313, and Synechococcus WH8102, located on contigs 26, 478 and 52, respectively, were obtained by consultation of the genome sequencing projects (http://www.jgi.doe.gov/JGI_microbial/html/prochlorococcus/prochlo_pickastrain.html and http://www.jgi.doe.gov/JGI_microbial/html/synechococcus/synech_homepage.html).
The GenBank accession numbers of additional 16S rDNA, ITS or 16S rDNAITS sequences used to investigate the specificity of primer 600 are as follows: Synechococcus PCC 6301, X00436; Synechocystis PCC 6803, D90916; Spirulina PCC 6313, X75045; Arthrospira PCC 8005, X70769; Arthrospira PCC 7345, X75044; environmental clone ENV WH7B, AJ007374; Spirulina subsalsa FACHB351, AF329394; all these sequences contain both the 16S rDNA and the ITS region. For the following strains two sequences were necessary to cover the 16S rDNAITS junction: Trichodesmium NIBB1067, X70767 (16S rDNA) and X72871 (ITS); Anabaena (Nostoc) PCC 7120, X59559 (16S rDNA) and AF180968 (ITS); Nodularia BCNOD 9427, AJ224447 (16S rDNA) and AJ224448 (ITS). For strains Pseudanabaena PCC 7403 and PCC 7409, and Chlorogloeopsis PCC 7518 (X687580; 16S rDNA), the 16S rDNA sequence and/or corresponding ITS were kindly provided by Gerard Van der Auwera and Annick Wilmotte (see also Iteman et al., 2000 ).
The sequences of the 16S rDNAITS junctions of Arthrospira OUQDS6 (AF329393), FACHB438 (AF329392) and FACHB439 (AF329391) are identical to that of Arthrospira PCC 7345 and, as for the corresponding sequence of Nostoc PCC 73102 (that shares 100% sequence identity in this domain with strain Anabaena PCC 7120), are not included in Fig. 4, but were counted in the total of 24 cyanobacterial 16S rDNAITS junctions compared (see Discussion). The 16S rDNA and ITS sequences of Nostoc PCC 73102 are both located on contig 647, available from the genome sequencing project (http://www.jgi.doe.gov/JGI_microbial/html/nostoc/nostoc_homepage.html).
Restriction endonuclease digestion of the ITS amplicons.
After amplification with primer pair 600 and 340, the PCR products (1020 µl) of the Prochlorococcus strains were digested with 5 U of the following restriction enzymes: AluI, DdeI, EcoRI, EcoRV, HaeIII, HinfI and HindIII (Gibco-BRL, Life Technologies), according to the instructions of the manufacturer. The DNA fragments were separated by electrophoresis for 46 h at 60 V on 2·5% (w/v) agarose gels (Metaphor, FMC, BioProducts) in 1x TBE buffer (Sambrook et al., 1989 ). Staining, DNA size markers and visualization of the restriction fragments were as described above.
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RESULTS |
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Amplification of the ITS region with primers 600 and 340
Given that the standard set of primers (322 and 340) amplified the ITS of the contaminants, forward primer 322 was replaced by primer 600, whose oligonucleotide sequence was designed on the basis of the 16S rDNA and ITS sequences of the axenic Prochlorococcus PCC 9511T (see below). Amplifications with this new set of primers performed on the axenic Prochlorococcus PCC 9511T and Synechococcus strains PCC 6307, PCC 7001 and WH7803 gave ITS amplicons of the expected size (compare Fig. 1a, b
; see also Table 2
). After subtraction of the 60 bp contributed by the end of the 16S rDNA (10 bp) and the beginning of the 23S rDNA (50 bp), the length of the ITS regions amounted, respectively, to about 540, 1000, 1050 and 820 bp, which is in good agreement with the estimates based on amplifications with primers 322 and 340 (Fig. 1a
). No additional bands were observed for the impure strain Synechococcus TAK RED (Fig. 1b
) and the non-axenic Prochlorococcus isolates (Table 2
), demonstrating the higher specificity of the new set of primers. Furthermore, PCR reactions performed at the same temperature (55 °C) as that used for the Prochlorococcus and Synechococcus strains, gave no amplicons with cells of the cyanobacterium Microcystis aeruginosa PCC 7941 and lysates of the bacterial strains isolated from the impure Prochlorococcus cultures (data not shown).
The sizes of the bands observed after amplification of the impure Prochlorococcus strains with primer set 600 and 340 (Table 2) were in accordance with those determined for the major PCR products obtained with primer pair 322 and 340 (Table 2
). Again it was possible to distinguish strains SS120 and NATL1-MIT from the other six Prochlorococcus isolates by their larger ITS size (about 640 versus 540 bp). The latter two strains correspond to members of the LL clade whereas, like the axenic strain PCC 9511T, four of the remaining five (NATL2, TAK 9803-2, GP2 and SB; Table 2
) are representatives of the HL clade (Urbach et al., 1998
; West & Scanlan, 1999
; West et al., 2001
; see also Table 2
). The phylogenetic position of strain OLI 36 FJA is unknown, but based on its ITS size (about 550 bp) would also be assignable to the HL clade. The size of the ITS of the impure strain of Synechococcus TAK RED (830 bp; see Fig. 1b
and Table 2
) proved again similar to that of the axenic Synechococcus WH7803 (820 bp; see Fig. 1a
, b
and Table 2
).
Restriction fragment length polymorphism (RFLP) of the ITS amplicons
The ITS amplicons of the seven non-axenic Prochlorococcus isolates and of the axenic strain PCC 9511 obtained with primer set 600 and 340 were digested with seven different restriction enzymes. Although no cutting sites could be identified for any of the ITS amplicons with the enzymes EcoRI, EcoRV and HindIII (not shown), RFLP was observed with the remaining four enzymes tested (Table 2). A representative gel of amplicons restricted with AluI is shown in Fig. 2
. Depending on the restriction enzyme employed, the RFLP patterns were composed of two to four bands between 70 and 500 bp (Table 2
) and it was possible to distinguish three RFLP subclusters (I.1, I.2A and I.2B) among the strains that yielded a small ITS amplicon (about 600 bp; Table 2
). Subcluster I.1 regroups the HLI strains PCC 9511T and NATL2 (West & Scanlan, 1999
; Rippka et al., 2000
) and includes OLI 36 FJA, whose phylogenetic position was previously unknown. Apart from fragments of short length (less than 70 bp) that were not detected (and thus the sum of the fragments may not add up perfectly to the size of the amplicons), the bands visualized by gel electrophoresis for the ITS amplicons of members of RFLP cluster I.1 are in good agreement with those expected on the basis of the restriction sites identified by DNA Strider 1.2 (Christian Marck, CEA, France) for the ITS sequence of Prochlorococcus MED4 (from the genome sequencing project) and that of Prochlorococcus PCC 9511T (see below). The latter analysis also confirmed the existence of restriction fragments of similar size (139 and 141 bp for AluI and 207 and 209 bp for HinfI) that are only revealed as a single band (doublets, Table 2
) of slightly stronger ethidium bromide fluorescence on the gels (see also Fig. 2
, after restriction of the amplicons with AluI).
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Sequences and alignments of the ITS
The sequences of the ITS regions were determined for Prochlorococcus PCC 9511T and two of the Synechococcus strains (PCC 6307 and PCC 7001). They were compared to those of Prochlorococcus MED4 and MIT9313, using as a reference the cyanobacterial ITS alignment proposed by Iteman et al. (2000) . In agreement with previous conclusions concerning the possible identity of strains Prochlorococcus PCC 9511T and MED4 (Rippka et al., 2000
), sequence comparison demonstrated that the ITS of these two strains are identical (data not shown). Consequently, the ITS sequence of strain MED4 was omitted from the alignment shown in Fig. 3
. For the reasons discussed below, the alignment also includes the last 10 nt of the 16S rRNA gene. This region, together with that covering the first 10 nt of the ITS, is fully conserved in all sequences compared (Fig. 3
), including MED4 (data not shown). In agreement with the approximate relative molecular mass determined for the ITS amplicons (see Fig. 1a
, b
and Table 2
), the ITS sequences for Prochlorococcus PCC 9511T (and MED4), Synechococcus PCC 6307 and PCC 7001 are 548, 1010 and 1065 bp in length, respectively. Strain Prochlorococcus MIT9313, a deeply branching member of the LL clade (Moore et al., 1998
; West & Scanlan, 1999
; West et al., 2001
), has an ITS of intermediate length (829 bp), compared to the two HLI strains Prochlorococcus PCC 9511T and MED4 and strains Synechococcus PCC 6307 and PCC 7001 (Fig. 3
), but is similar in size to the ITS of 820 and 830 bp determined, respectively, for the oceanic Synechococcus strains WH7803 (Fig. 1a
, b
; Table 2
) and TAK RED (Fig. 1b
; Table 2
).
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In spite of the differences in size and base composition, as well as extensive sequence divergence in the more variable regions of the four ITS sequences aligned, common conserved domains, such as the two tRNA genes (encoding tRNAIle and tRNAAla), could be identified (Fig. 3) and also include box A and motifs D1, D1' and D4 (Fig. 3
), the former being important for transcriptional antitermination, the latter three for folding of the rRNA transcripts (Iteman et al., 2000
).
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DISCUSSION |
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In contrast to filamentous cyanobacteria that often have more than one rrn operon with ITS regions of at least two different sizes (Lu et al., 1997 ; West & Adams, 1997
; Neilan et al., 1997
; Iteman et al., 1999
, 2000
; Barker et al., 1999
), a single ITS amplicon was observed for all strains of Prochlorococcus and Synechococcus. This may suggest that, like in the genomes of Prochlorococcus MED4 and MIT9313 and the oceanic Synechococcus WH8102, a single rrn operon exists in all the strains examined here. However, it is also possible that, at least in some of these isolates, more than one copy of the rrn operon is present in their genome, but that the corresponding ITS regions are identical or very similar in size, as is the case for the unicellular cyanobacteria Synechococcus PCC 6301 and Synechocystis PCC 6803, both of which have two nearly identical ITSs (Williamson & Doolittle, 1983
; Tomioka & Sugiura, 1984
; Iteman et al., 2000
). If multiple rrn copies exist in the genomes of the strains of Prochlorococcus examined, both the sizes and recognition sequences of their ITS seem to be identical, since the sums of the restriction fragments are in fair agreement with the lengths of the ITS amplicons (Table 2
) and not larger, as would be the case if there were sequence variations in the recognition sites.
The groupings obtained by RFLP of the ITS amplicons for the eight strains of Prochlorococcus examined, correlated well with the three different genotypes (HLI, HLII and LL) recognized on the basis of 16S rRNA gene sequences (Urbach et al., 1998 ; West & Scanlan, 1999
; Rippka et al., 2000
; West et al., 2001
) and other molecular characterizations (Scanlan et al., 1996
; Urbach et al., 1998
; West & Scanlan, 1999
; West et al., 2001
). This clearly demonstrates the overall value of this simple technique. However, it was not possible to discriminate between the two LL representatives SS120 and NATL1-MIT, although, based on 16S rDNA analyses, they are slightly more distant from one another than are the more interrelated HLI and HLII strains (Urbach et al., 1998
; West & Scanlan, 1999
; West et al., 2001
). Thus, for a higher level of discrimination between these two LL strains, analyses with a wider range of restriction enzymes or ITS sequence information will be required. The low degree of divergence in the 16S rRNA genes between the most distantly related HL and LL representatives of Prochlorococcus (97·3% similarity; West et al., 2001
), suggests that the three RFLP groupings (I.1, I.2A and I.2B) obtained for the HL strains may correspond to distinctions at the subspecies level. In contrast, the larger ITS size and different RFLP profiles observed for the two LL strains, compared to all HL isolates, would be consistent with them being members of a different species. However, confirmation of these postulated taxonomic relationships needs to await DNADNA hybridization studies.
Analyses of the region covering the last 10 bp in the 16S rRNA gene and the first 10 bp in the ITS for a total of 24 cyanobacteria, for which this sequence information is presently available (see Methods), revealed the specificity of the new primer 600. As shown in Fig. 4, only Prochlorococcus PCC 9511, MED4 and MIT9313, and strains PCC 6307, PCC 7001 and the oceanic Synechococcus WH8102 show 100% sequence identity within the complementary target domain. For all other cyanobacteria, three or more mismatches could be identified (Fig. 4
) and, as experimentally confirmed for the randomly chosen cyanobacterium Microcystis aeruginosa PCC 7941, are sufficient to prevent PCR amplification, if using an annealing temperature of 55 °C. Consequently, with this new group-specific primer the ITS region can be selectively amplified from Prochlorococcus and all Synechococcus strains of the OMF-Synechococcus clade, even if the cultures are contaminated by several different bacteria. The latter is particularly important for the genus Prochlorococcus, since only a single axenic strain (PCC 9511T) of this genus is presently available (Rippka et al., 2000
).
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In spite of differences in size and mean DNA base composition, comparison of the new ITS sequences of Prochlorococcus PCC 9511T and the two Synechococcus strains (PCC 6307 and PCC 7001) with those of Prochlorococcus MIT9313 (Fig. 3) and MED4 (data not shown), revealed valuable insights. Several conserved domains important either for transcriptional antitermination (box A) or folding (the complementary domains D1 and D1' close to the 5' end of the ITS, together with domain D4 immediately adjacent to box A) of the rRNA transcripts were identified as in other cyanobacteria (Iteman et al., 2000
) and two tRNA genes encoding tRNAIle and tRNAAla were found for all strains. This is in contrast to some other cyanobacterial ITSs that may lack one or both tRNA genes (Iteman et al., 2000
). As in most other cyanobacterial ITS regions (Iteman et al., 2000
), both tRNA genes lack the 3'-terminal CCA extension found in many bacteria, although they contain the characteristic subterminal CCA sequence that appears to be typical of cyanobacteria (Iteman et al., 2000
). The overall sequence similarity of the ITS sequences, including some of the more variable domains, was also higher among these five strains than that observed with respect to the ITS of other cyanobacterial genera (compare Fig. 3
with Fig. 3
of Iteman et al., 2000
). However, major differences in sequence are evident in certain regions. Prochlorococcus MIT9313 differs from strain PCC 9511 in possessing a long insert (positions 8831001; Fig. 3
) and 12 short inserts situated throughout the ITS. These inserts are also observed in Synechococcus strains PCC 6307 and PCC 7001, although the latter organisms differ in the positions of additional inserts that further increase the length of their ITS regions beyond that of strain MIT9313: the most significant of these start at alignment positions 44, 64, 181, 258, 304, 336, 589, 746 and 1116 for PCC 6307, and at 138, 157, 258, 304, 443, 556, 649, 691, 1078 and 1132 for PCC 7001. Since strains PCC 6307 and PCC 7001 differ markedly in sequence in certain regions, similar ITS sizes do not necessarily indicate close genetic relationships. However, in the case of Prochlorococcus MIT9313 and the oceanic Synechococcus strain WH7803, for which the phylogenetic relationship is known (West et al., 2001
), the similarity in length of this domain may be of significance. Indeed, in 16S rRNA gene trees, strain MIT9313 together with Prochlorococcus MIT9303, occupies a position that forms the root of the LL Prochlorococcus clade and is closest to the oceanic cluster of the OMF-Synechococcus clade (West et al., 2001
).
The availability of the three new ITS sequences, together with those of Prochlorococcus MED4 and MIT9313, should permit the design of new primers that, in combination with the group-specific primer set 600 and 340, may be used to achieve identification of strains or field samples at different resolution (i.e. at a lower or higher taxonomic rank) by PCR. In addition, probes complementary to discriminatory regions of the ITS may also be designed and labelled to attempt single-cell hybridization and detection by light microscopy or flow cytometry, possibly resulting in a higher specificity of identification than is presently achieved with probes targeting the more conserved 16S rRNA molecule (West et al., 2001 ; Worden et al., 2000
). However, the search for such specific primers or probes will profit from the determination of additional ITS sequences. Finally, as more complete 16S and 23S rRNA gene and ITS sequences become available, secondary structure analyses will provide valuable insights into evolutionary aspects of these domains in the ribosomal operon of cyanobacteria from oceanic, marine and freshwater environments.
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ACKNOWLEDGEMENTS |
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REFERENCES |
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Received 28 June 2001;
revised 21 September 2001;
accepted 2 October 2001.