- Email: [email protected]
Application of the variable region in 16S rDNA to create an index for rapid species identification in the genus Streptomyces
FEMS Microbiology Letters 151 (1997) 249^255
Application of the variable region in 16S rDNA to create an index for rapid species identi¢cation in the genus Streptomyces Masakazu Kataoka b
1 ;2 ;a
, Kumiko Ueda 3 a , Takuji Kudo b , Tatsuji Seki a *, Toshiomi Yoshida a ;
;
a The International Center for Biotechnology, Osaka University, Yamada-oka, Suita, Osaka 565, Japan Japan Collection of Microorganisms, Institute of Physical and Chemical Research (RIKEN), Hirosawa, Wako, Saitama 351-01, Japan
Received 10 April 1997 ; accepted 14 April 1997
Abstract
Partial nucleotide sequences (120 bp) of the 16S rRNA gene (rDNA) containing a variable K region were compared in 89 strains of the genus Streptomyces belonging to eight major clusters of category I in Bergey's Manual of Systematic Bacteriology. Fifty-seven kinds of partial 16S rDNA sequences were observed among the 89 strains. Forty-three of the strains were grouped into 11 `identity groups', based on the fact that the strains in each group shared an identical sequence in the 120bp region. The results of a phylogenetic analysis based on the 16S rDNA 120-bp sequences revealed that 60 of the 89 strains could be categorized into seven clusters, each consisting of four or more strains. Based on these observations it was concluded that short nucleotide sequences bearing the variable K region are useful for Streptomyces species identification. Keywords : Phylogenetic analysis; Streptomyces; 16S rRNA gene
1. Introduction
In the conventional taxonomy of Streptomyces, its systematics is, in practice, based on characteristics of mycelial morphology, pigment production, and cer* Corresponding author. Tel.: +81 (6) 8797453; fax: +81 (6) 8797454; e-mail: [email protected] 1
M. Kataoka and K. Ueda contributed equally to this work.
2 Present address: Mitsubishi-Kasei Institute of Life Sciences, 11 Minami-Ooya, Machida-shi, Tokyo 194, Japan. 3 Present address: Institute for Fermentation, Osaka, Juso-honmachi,Yodogawa-ku, Osaka 532, Japan.
tain physiological properties. In 1964, the International Streptomyces Project (ISP), a collaborative study group on Streptomyces taxonomy, proposed an elaborate description of criteria for some of the authentic and extant type strains of Streptomyces and their related taxa, which is dependent on a limited number of taxonomic characteristics selected from those accumulated in conventional taxonomic tests [1,2]. In 1983, a large-scale numerical phenetic survey of Streptomyces and related taxa was carried out by Williams et al. [3]; 394 strains of Streptomyces-type cultures were examined with respect to 139 taxonomic characteristics and the results were analyzed statistically. Based on the ¢ndings, Streptomy-
0378-1097 / 97 / $17.00 ß 1997 Federation of European Microbiological Societies. Published by Elsevier Science B.V. PII S 0 3 7 8 - 1 0 9 7 ( 9 7 ) 0 0 1 6 9 - 9
FEMSLE 7597 2-9-97
250
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
-type strains were grouped into 23 `major clusters' each containing four or more strains, 20 `minor clusters' each containing two to three strains, and 25 `single member clusters' [3]. The results of the above work are compiled in a chapter of Bergey's Manual of Systematic Bacteriology, Vol. 4 [4]. The proposed classi¢cation, however, disagrees with that obtained by the conventional taxonomic methods in several respects. Recent progress in molecular biology and population genetics has dramatically increased the amount of evolutionary information available for species classi¢cation. For example, a database of ribosomal RNA genes, particularly of small subunits of ribosomal RNAs (16S rRNAs), has been compiled and successfully applied to determining phylogenetic relationships in bacteria [5]. In the case of Streptomyces, these studies have revealed that, in some cases, phenetic classi¢cation better re£ects the phylogenetic relationships between the strains examined [6,7]. Here, 89 ISP standard strains belonging to eight major clusters of category I de¢ned by numerical identi¢cation in Bergey's Manual of Systematic Bacteriology [4] were subjected to a sequence comparison of a part of their 16S rRNA gene containing a highly variable K region and to phylogenetic analysis. From the phylogenetic relationships of these strains, we propose the usefulness of a data base generated on the basis of partial rDNA sequences for the rapid identi¢cation of species of the genus Streptomyces. ces
2. Materials and methods
2.1. Strains and culture conditions
The 89 strains of the genus Streptomyces used in this study (see Fig. 3) were obtained from the Japan Culture Collection of Microorganisms (JCM; Riken, Wako, Saitama, Japan). All these strains belong to eight major clusters (species groups) of category I, de¢ned by numerical classi¢cation, in Bergey's Manual of Systematic Bacteriology [4]: S. albido£avus, S. anulatus, S. halstedii, S. exfoliatus, S. violaceus, S. fulvissimus, S. rochei and S. chromofuscus
. They were cultivated by the methods recommended in the JCM Strain Catalogue [8].
2.2. PCR ampli¢cation and sequencing of a part of 16S rDNA
To achieve the reliable sequencing of the partial 16S rDNA obtained by PCR ampli¢cation from various Streptomyces strains, direct sequencing of PCR products were carried out. Chromosomal DNA for the PCR template was prepared from cells in a single colony formed on a plate using an Insta Gene kit (Bio-Rad) according to the supplier's protocol. DNA fragments covering the variable region of 16S rDNA was ampli¢ed using phosphorylated sense and nonphosphorylated anti-sense primers [10]. The sense primer was phosphorylated using T4 polynucleotide kinase (Takara Shuzo) and ATP. PCR was performed in 50 Wl reaction mixture (10 mM Tris-HCl, pH 8.3; 50 mM KCl; 1.5 mM MgCl2 ; 0.001%, w/v, glycerol) for 30 or 40 cycles of denaturation (for 30 s at 97³C), annealing (for 1 min at 50³C) and extension (for 1 min at 72³C) with Amplitaq DNA polymerase (Perkin Elmer). Whole samples were fractionated by agarose gel electrophoresis, and PCR products of 500 bp were recovered using a Gene Clean II kit (Bio 101). The phosphorylated sense strand was digested for 1 h at 37³C with V-exonuclease (BRL) in the recommended bu¡er (67 mM glycine-KOH, pH 9.4; 2.5 mM MgCl2 [9]). After phenol/chloroform extraction, the remaining antisense strand was used as a sequencing template. DNA sequences were determined using a 7-deaza dGTP Sequenase Version 2.0 kit (USB) according to the supplier's protocol, except that 1 Wg of singlestranded DNA binding protein (SSB, Stratagene) was added to 15 Wl of the reaction mixture. After termination of the reaction, SSB was digested with 20 Wg proteinase K (Sigma) for 30 min at 37³C in 6 Wl of the termination mixture. 2.3. Oligonucleotides
Nucleotide sequences of the synthesized oligonucleotides used were as follows. Sense primer for PCR: 5P-TCACGGAGAGTTTGATCCTG-3P ; anti-sense primer for PCR: 5P-GCGGCTGCTGGCACGTAGTT-3P ; sequencing primer: 5P-AGTAACACGTGGGCAATCTG-3P. The primer sequences were selected from the conserved region and corresponded to nucleotide positions 1^20, 481^500, and 105^124, re-
FEMSLE 7597 2-9-97
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
Fig. 1. Phylogenetic relationships among published nucleotide sequences of the 16S rRNA gene in seven
251
Streptomyces
strains. The phylo-
genetic trees were constructed by the neighbor-joining method using whole (left) and partial (right) sequences of the 16S rRNA gene. The bar labeled 0.05 indicates 5 base changes per 100 nucleotides.
spectively, according to the
ciens
Streptomyces ambofa-
rDNA sequence [11].
estimated by the method of Kimura [12]. The phylogenetic tree was constructed by the neighbor-joining method [13].
2.4. Analysis of rDNA sequences and construction of phylogenetic trees 3. Results and discussion
Nucleotide sequences of the ampli¢ed products were edited by the GENETYX program (Software Development)
on
a
PC9801
personal
computer
(NEC). Evolutionary analysis of nucleotide sequen-
3.1. Selection of a variable region suitable for phylogenetic analysis in the 16S rRNA gene of Streptomyces
ces was performed using the ODEN program (National Institute of Genetics, Japan). For construction
To identify the most informative region of 16S
Streptomyces
of the evolutionary genetic distance matrices, fre-
rDNAs for the phylogenetic study of
quencies of base substitutions per nucleotide were
species, the nucleotide sequences of 16S rDNAs of
Fig. 2. Sequence variation in the variable region of 16S rRNA among 17 corresponding to the 16S rRNA gene of
S. ambofaciens.
Streptomyces
strains. Numerals indicate the nucleotide positions
The region of nucleotide positions 172^202 is the most variable region, and is be-
lieved to form a stem and loop structure (see text). Asterisks represent perfectly conserved bases in the 17 species so far examined.
FEMSLE 7597 2-9-97
252
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
FEMSLE 7597 2-9-97
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255 Fig. 3. Phylogenetic tree constructed from the 120-bp
K
region sequences of 89
Streptomyces
253
strains belonging to eight major clusters of
category I in Bergey's Manual of Systematic Bacteriology [4]. Strain names are followed by the description in JCM catalogue but are cited as subjective synonyms in Bergey's Manual except for the type strains of the major cluster. The number preceding the species name indicates a major cluster of category I used in Bergey's manual : 1,
olaceus ;
6,
S. fulvissimus ;
S. rochei ;
7,
cession numbers (D) for the 120-bp
6
K
8,
S. chromofuscus.
S. albido£avus ;
S. anulatus ;
2,
3,
S. halstedii;
4,
S. exfoliatus ;
5,
S. vi-
JCM strain numbers (J), ISP strain numbers (I) and DDBJ DNA sequence ac-
region sequences are given along with the strain names. The IG and PC group symbols are shown
in bold letters. The bar labeled 0.05 indicates 5 base changes per 100 nucleotides.
Streptomyces lividans S. griseus [16],
[15],
S. coelicolor A3(2) S. ambofaciens [11] were
TK21 [14],
nucleotides in the stem were changed together. The
and
GCAT sequence in the loop was found to be highly
aligned. This enabled the selection of a 120-bp region
conserved, indicating that it may have an important
from nucleotide positions 158^277 of the 16S rRNA
role in the ribosome function. Only three strains,
S. ambofaciens,
gene of iable
K
as it includes the most var-
region [17].
To test the verity of a phylogenetic tree based on partial sequences of the 16S rRNA gene, we compared
two
phylogenetic
trees
constructed
by
alboniger (Fig. spheroides (not having
a
S. niveus
2),
(not
shown),
and
S. S.
shown), di¡ered from the others in
TCCT
sequence
at
the
corresponding
GCAT site.
the
Among the 89 strains, 57 kinds of 120-bp nucleo-
neighbor-joining method using published total and
tide sequences could be identi¢ed. In particular, 11
Streptomyces
identical sequences were shared by 47 of the strains :
strains [11,14^16,18]. We found the general topolo-
each sequence was shared by two to eight strains.
gies of the trees from the partial and total sequences
The groups containing these strains were designated
to be similar (Fig. 1), but the genetic distance to be
as `identity groups' (IGs). It is apparent from Fig. 3
more emphasized in the partial-sequence tree. This
that the strains in each IG belong to the same re-
observation indicated that the variation in the partial
spective numerical major cluster, the only exception
16S rDNA sequences covering the variable region is
being IG-G which includes strains from the major
su¤cient for deducing phylogenetic relationships of
clusters of
Streptomyces
fact
partial 16S rRNA sequences of seven
strains
at
the
intra-species
level,
that
S. exfoliatus
K
the
region
and is
S. violaceus.
the
most
From the
variable,
it
is
although these segments are probably too variable
thought that strains labeled as various di¡erent spe-
for comparison at the generic level.
cies names but sharing an identical sequence may actually belong to a single species even though minor
3.2. DNA sequences of 89 independent Streptomyces strains A 500-bp DNA sequence, partially encompassing the
16S
sample
rRNA
gene,
prepared
was
from
a
ampli¢ed
single
from
colony
of
a
DNA
each
in
K region was determined (see Fig. 3 for the
nucleotide
assisted
the
hyper-variable
characteristics
re-
To clarify the phylogenetic relationships of the 89
Streptomyces the variable
of
phenotypic
3.3. Phylogenetic relationship through the partial sequence
DDBJ accession numbers of these sequences). The sequences
their
sulted in their being classi¢ed as di¡erent.
of
the 89 strains, and the 120-bp sequence bearing the variable
di¡erences
region
strains, the 120-bp sequences bearing
K
region were subjected to computer-
phylogenetic
analysis
for
the
construction
from nucleotide positions 172^202 in 17 out of the
of a phylogenetic tree (Fig. 3). This tree has seven
89 strains, as well as some variations outside of the
major
region, are shown in Fig. 2. It has been suggested
PC-G), each comprised of four or more strains ; 60
that the hyper-variable region forms a stem and loop
of the 89 strains were classi¢ed into these seven clus-
structure in vivo in
S. ambofaciens
16S rRNA [11].
phylogenetic
clusters
(classi¢ed
as
PC-A
to
ters. Williams et al. [3] have shown that the numer-
S. albido£avus, S. anulatus, and S.
The conservation of the secondary structure is par-
ical major clusters,
ticularly notable, but the sequences forming the stem
halstedii,
are the most variable : the most of complementing
to form a large `super cluster'. This is partially in line
FEMSLE 7597 2-9-97
are closely related, and can be considered
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
254
with our results, the exception being the strains of the
S. albido£avus major cluster ;
according to the
phylogenetic tree generated (Fig. 3), these are not closely related to the strains belonging to the major
S. anulatus, and S. halstedii. In our tree, strains of the S. albido£avus major cluster are
clusters of all the
grouped
into
phylogenetic
cluster
PC-D
with
less
than three base substitutions. The homogeneity of these strains has also been suggested by the results
of type cultures of
Streptomyces. IV. Species descriptions from
the second, third and fourth studies. Int. J. Syst. Bacteriol. 19, 391^512. [2] Shirling, E.B. and Gottlieb, D. (1972) Cooperative description of type strains of
Streptomyces.
V. Additional descriptions.
Int. J. Syst. Bacteriol. 22, 265^394. [3] Williams,
S.T.,
Goodfellow,
M.,
Alderson,
G.,
Wellington,
E.M.H., Sneath, P.H.A. and Sackin, M.J. (1983) Numerical classi¢cation of
Streptomyces
and related genera. J. Gen. Mi-
crobiol. 129, 1743^1813. [4] Williams, S.T., Goodfellow, M. and Alderson, G. (1989) Ge-
Streptomyces
AL .
from whole 16S rRNA sequences [19], chromosomal
nus
DNA hybridization [20], pyrolysis mass spectrometry
Bergey's Manual of Systematic Bacteriology, Vol. 4 (S.T. Wil-
[21] and fatty acid analysis [22]. PC-B is the largest cluster in our tree, comprising 19 of the 25 strains of the
S. anulatus major cluster and ¢ve of the seven S. halstedii major cluster but it is not
strains of the
closely related to PC-D. Strains of other numerical cluster
were
found
to
be
distributed among
other
phylogenetic clusters or were independent. The identity groups IG-J and IG-K are closely related to PCG. The two strains belonging to IG-K,
S. £aviscle-
rotiacus and S. minutisclerotiacus, were formerly classi¢ed as Chainia species, but were later transferred to Streptomyces [23].
Waksman
and
Henrici,
1943,
339
In :
liams, M.E. Sharpe and J.G. Holt, Eds.), pp. 2452^2492. Williams and Wilkins, Baltimore, MD. [5] Woese, C.R. (1987) Bacterial evolution. Microbiol. Rev. 51, 221^271. [6] Gladek, A., Mordarski, A., Goodfellow, M. and Williams, S.T. (1985) Ribosomal ribonucleic acid similarities in the classi¢cation of
Streptomyces.
FEMS Microbiol. Lett. 26, 175^
180. [7] Witt, D. and Stackebrandt, E. (1990) Uni¢cation of the gen-
Streptoverticillum and Streptomyces, and amendation of Streptomyces Waksman and Henrici 1943, 339AL . Syst. era
Appl. Microbiol. 13, 361^371. [8] Nakase, T. (1992) In : JCM Catalogue of Strains, 5th edn. (T. Nakase, Ed.), RIKEN, Saitama, Japan. [9] Higuchi,
R.G.
and
Ochman,
H.
(1989)
Production
of
In conclusion, we believe that the phylogenetic tree
single-stranded DNA templates by exonuclease digestion fol-
presented here will serve as a useful tool for rapid
lowing the polymerase chain reaction. Nucleic Acids Res. 17,
identi¢cation
of
newly isolated
the
phylogenetic
Streptomyces
localization
of
strains, and that it is
likely to prove more e¡ective than the conventional methods. Additionally, it should provide a means for
5865. [10] Saiki, R.K., Gelfand, D.H., Sto¡e, S., Scharf, S.J., Higuchi, R., Horn, G.T., Mullis, K.B. and Erlich, H.A. (1988) Primerdirected enzymatic ampli¢cation of DNA with a thermostable DNA polymerase. Science 239, 487^491.
easy and appropriate identi¢cation, which is espe-
[11] Pernodet, L.L., Boccard, F., Alegre, M.T., Gagnat, J. and
cially important in the fermentation industry in or-
è rineau, M. (1989) Organization and nucleotide sequence Gue
der to avoid taxonomic confusion of strains dealt with in patent literature.
analysis of a ribosomal RNA gene cluster from
ambofaciens.
Streptomyces
Gene 79, 33^46.
[12] Kimura, M. (1980) A simple method for estimating evolutionary rates of base substitutions through comparative studies of nucleotide sequences. J. Mol. Evol. 16, 111^120.
Acknowledgments We
are
[13] Saitou, N. and Nei, M. (1987) The neighbor-joining method : a
grateful
to
Tobias
Kieser
(John
Innes
new
method
for
16S
partially
Acids Res. 16, 370.
T.Y.
under
the
by
Grant-in
International
Aid
07044149
Scienti¢c
to
Research
Project of the Japanese Ministry of Science, Educa-
phylogenetic
trees.
Mol.
[14] Suzuki, Y. and Yamada, T. (1988) The nucleotide sequence of
Centre, UK) for helpful discussions. This work was supported
reconstructing
Biol. Evol. 4, 406^425.
rRNA gene from
Streptomyces lividans
TK21. Nucleic
[15] Baylis, H.A. and Bibb, M.J. (1989) The nucleotide sequence of a 16S rRNA gene from
Streptomyces coelicolor
A3(2). Nucleic
Acids Res. 18, 831.
tion, Sports and Culture.
[16] Kim, E., Kim, H., Kang, K.H., Kho, Y.H. and Park, Y.-H. (1991) Complete nucleotide sequence of a 16S ribosomal RNA
References
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Streptomyces griseus
subsp.
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[1] Shirling, E.B. and Gottlieb, D. (1969) Cooperative description
and
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Liesack,
W.
(1991)
Designation
of
streptomycetes
16S
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(G.
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and 23S rRNA-based target regions of oligonucleotide probes.
of
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Eds.), pp. 517^525. Akademiai Kiado, Budapest.
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S.
Biro
and
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[18] Mehling, A., Wehmeier, U.F. and Piepersberg, W. (1995) Nu-
[21] Sanglier, J.-J., Whitehead, D., Saddler, G.S., Ferguson, E.V.
cleotide sequences of streptomycete 16S ribosomal DNA : to-
and Goodfellow, M. (1992) Pyrolysis mass spectrometry as a
wards a speci¢c identi¢cation system for streptomycetes using
method for the classi¢cation, identi¢cation and selection of actinomycetes. Gene 115, 235^242.
PCR. Microbiology 141, 2139^2147. [19] Kampfer,
P.,
Kroppenstedt,
R.M.
and
numerical classi¢cation of the genera
toverticillum
using
miniaturized
Dott,
W.
Streptomyces
physiological
A
[22] Saddler, G.S., O'Donnell, A.G., Goodfellow, M. and Minni-
Strep-
kin, D.E. (1987) SIMCA pattern recognition in the analysis of
(1991) and
tests.
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Gen.
[20] Mordarski, M., Goodfellow, M., Williams, S.T. and Sneath, P.H.A. (1986) Evaluation of species groups in the genus
tomyces.
streptomycetes fatty acids. J. Gen. Microbiol. 133, 1137^1147. [23] Goodfellow,
Microbiol. 137, 1831^1891.
Strep-
In : Biological, Biochemical and Biomedical Aspects
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FEMSLE 7597 2-9-97
Application of the variable region in 16S rDNA to create an index for rapid species identi¢cation in the genus Streptomyces Masakazu Kataoka b
1 ;2 ;a
, Kumiko Ueda 3 a , Takuji Kudo b , Tatsuji Seki a *, Toshiomi Yoshida a ;
;
a The International Center for Biotechnology, Osaka University, Yamada-oka, Suita, Osaka 565, Japan Japan Collection of Microorganisms, Institute of Physical and Chemical Research (RIKEN), Hirosawa, Wako, Saitama 351-01, Japan
Received 10 April 1997 ; accepted 14 April 1997
Abstract
Partial nucleotide sequences (120 bp) of the 16S rRNA gene (rDNA) containing a variable K region were compared in 89 strains of the genus Streptomyces belonging to eight major clusters of category I in Bergey's Manual of Systematic Bacteriology. Fifty-seven kinds of partial 16S rDNA sequences were observed among the 89 strains. Forty-three of the strains were grouped into 11 `identity groups', based on the fact that the strains in each group shared an identical sequence in the 120bp region. The results of a phylogenetic analysis based on the 16S rDNA 120-bp sequences revealed that 60 of the 89 strains could be categorized into seven clusters, each consisting of four or more strains. Based on these observations it was concluded that short nucleotide sequences bearing the variable K region are useful for Streptomyces species identification. Keywords : Phylogenetic analysis; Streptomyces; 16S rRNA gene
1. Introduction
In the conventional taxonomy of Streptomyces, its systematics is, in practice, based on characteristics of mycelial morphology, pigment production, and cer* Corresponding author. Tel.: +81 (6) 8797453; fax: +81 (6) 8797454; e-mail: [email protected] 1
M. Kataoka and K. Ueda contributed equally to this work.
2 Present address: Mitsubishi-Kasei Institute of Life Sciences, 11 Minami-Ooya, Machida-shi, Tokyo 194, Japan. 3 Present address: Institute for Fermentation, Osaka, Juso-honmachi,Yodogawa-ku, Osaka 532, Japan.
tain physiological properties. In 1964, the International Streptomyces Project (ISP), a collaborative study group on Streptomyces taxonomy, proposed an elaborate description of criteria for some of the authentic and extant type strains of Streptomyces and their related taxa, which is dependent on a limited number of taxonomic characteristics selected from those accumulated in conventional taxonomic tests [1,2]. In 1983, a large-scale numerical phenetic survey of Streptomyces and related taxa was carried out by Williams et al. [3]; 394 strains of Streptomyces-type cultures were examined with respect to 139 taxonomic characteristics and the results were analyzed statistically. Based on the ¢ndings, Streptomy-
0378-1097 / 97 / $17.00 ß 1997 Federation of European Microbiological Societies. Published by Elsevier Science B.V. PII S 0 3 7 8 - 1 0 9 7 ( 9 7 ) 0 0 1 6 9 - 9
FEMSLE 7597 2-9-97
250
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
-type strains were grouped into 23 `major clusters' each containing four or more strains, 20 `minor clusters' each containing two to three strains, and 25 `single member clusters' [3]. The results of the above work are compiled in a chapter of Bergey's Manual of Systematic Bacteriology, Vol. 4 [4]. The proposed classi¢cation, however, disagrees with that obtained by the conventional taxonomic methods in several respects. Recent progress in molecular biology and population genetics has dramatically increased the amount of evolutionary information available for species classi¢cation. For example, a database of ribosomal RNA genes, particularly of small subunits of ribosomal RNAs (16S rRNAs), has been compiled and successfully applied to determining phylogenetic relationships in bacteria [5]. In the case of Streptomyces, these studies have revealed that, in some cases, phenetic classi¢cation better re£ects the phylogenetic relationships between the strains examined [6,7]. Here, 89 ISP standard strains belonging to eight major clusters of category I de¢ned by numerical identi¢cation in Bergey's Manual of Systematic Bacteriology [4] were subjected to a sequence comparison of a part of their 16S rRNA gene containing a highly variable K region and to phylogenetic analysis. From the phylogenetic relationships of these strains, we propose the usefulness of a data base generated on the basis of partial rDNA sequences for the rapid identi¢cation of species of the genus Streptomyces. ces
2. Materials and methods
2.1. Strains and culture conditions
The 89 strains of the genus Streptomyces used in this study (see Fig. 3) were obtained from the Japan Culture Collection of Microorganisms (JCM; Riken, Wako, Saitama, Japan). All these strains belong to eight major clusters (species groups) of category I, de¢ned by numerical classi¢cation, in Bergey's Manual of Systematic Bacteriology [4]: S. albido£avus, S. anulatus, S. halstedii, S. exfoliatus, S. violaceus, S. fulvissimus, S. rochei and S. chromofuscus
. They were cultivated by the methods recommended in the JCM Strain Catalogue [8].
2.2. PCR ampli¢cation and sequencing of a part of 16S rDNA
To achieve the reliable sequencing of the partial 16S rDNA obtained by PCR ampli¢cation from various Streptomyces strains, direct sequencing of PCR products were carried out. Chromosomal DNA for the PCR template was prepared from cells in a single colony formed on a plate using an Insta Gene kit (Bio-Rad) according to the supplier's protocol. DNA fragments covering the variable region of 16S rDNA was ampli¢ed using phosphorylated sense and nonphosphorylated anti-sense primers [10]. The sense primer was phosphorylated using T4 polynucleotide kinase (Takara Shuzo) and ATP. PCR was performed in 50 Wl reaction mixture (10 mM Tris-HCl, pH 8.3; 50 mM KCl; 1.5 mM MgCl2 ; 0.001%, w/v, glycerol) for 30 or 40 cycles of denaturation (for 30 s at 97³C), annealing (for 1 min at 50³C) and extension (for 1 min at 72³C) with Amplitaq DNA polymerase (Perkin Elmer). Whole samples were fractionated by agarose gel electrophoresis, and PCR products of 500 bp were recovered using a Gene Clean II kit (Bio 101). The phosphorylated sense strand was digested for 1 h at 37³C with V-exonuclease (BRL) in the recommended bu¡er (67 mM glycine-KOH, pH 9.4; 2.5 mM MgCl2 [9]). After phenol/chloroform extraction, the remaining antisense strand was used as a sequencing template. DNA sequences were determined using a 7-deaza dGTP Sequenase Version 2.0 kit (USB) according to the supplier's protocol, except that 1 Wg of singlestranded DNA binding protein (SSB, Stratagene) was added to 15 Wl of the reaction mixture. After termination of the reaction, SSB was digested with 20 Wg proteinase K (Sigma) for 30 min at 37³C in 6 Wl of the termination mixture. 2.3. Oligonucleotides
Nucleotide sequences of the synthesized oligonucleotides used were as follows. Sense primer for PCR: 5P-TCACGGAGAGTTTGATCCTG-3P ; anti-sense primer for PCR: 5P-GCGGCTGCTGGCACGTAGTT-3P ; sequencing primer: 5P-AGTAACACGTGGGCAATCTG-3P. The primer sequences were selected from the conserved region and corresponded to nucleotide positions 1^20, 481^500, and 105^124, re-
FEMSLE 7597 2-9-97
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
Fig. 1. Phylogenetic relationships among published nucleotide sequences of the 16S rRNA gene in seven
251
Streptomyces
strains. The phylo-
genetic trees were constructed by the neighbor-joining method using whole (left) and partial (right) sequences of the 16S rRNA gene. The bar labeled 0.05 indicates 5 base changes per 100 nucleotides.
spectively, according to the
ciens
Streptomyces ambofa-
rDNA sequence [11].
estimated by the method of Kimura [12]. The phylogenetic tree was constructed by the neighbor-joining method [13].
2.4. Analysis of rDNA sequences and construction of phylogenetic trees 3. Results and discussion
Nucleotide sequences of the ampli¢ed products were edited by the GENETYX program (Software Development)
on
a
PC9801
personal
computer
(NEC). Evolutionary analysis of nucleotide sequen-
3.1. Selection of a variable region suitable for phylogenetic analysis in the 16S rRNA gene of Streptomyces
ces was performed using the ODEN program (National Institute of Genetics, Japan). For construction
To identify the most informative region of 16S
Streptomyces
of the evolutionary genetic distance matrices, fre-
rDNAs for the phylogenetic study of
quencies of base substitutions per nucleotide were
species, the nucleotide sequences of 16S rDNAs of
Fig. 2. Sequence variation in the variable region of 16S rRNA among 17 corresponding to the 16S rRNA gene of
S. ambofaciens.
Streptomyces
strains. Numerals indicate the nucleotide positions
The region of nucleotide positions 172^202 is the most variable region, and is be-
lieved to form a stem and loop structure (see text). Asterisks represent perfectly conserved bases in the 17 species so far examined.
FEMSLE 7597 2-9-97
252
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
FEMSLE 7597 2-9-97
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255 Fig. 3. Phylogenetic tree constructed from the 120-bp
K
region sequences of 89
Streptomyces
253
strains belonging to eight major clusters of
category I in Bergey's Manual of Systematic Bacteriology [4]. Strain names are followed by the description in JCM catalogue but are cited as subjective synonyms in Bergey's Manual except for the type strains of the major cluster. The number preceding the species name indicates a major cluster of category I used in Bergey's manual : 1,
olaceus ;
6,
S. fulvissimus ;
S. rochei ;
7,
cession numbers (D) for the 120-bp
6
K
8,
S. chromofuscus.
S. albido£avus ;
S. anulatus ;
2,
3,
S. halstedii;
4,
S. exfoliatus ;
5,
S. vi-
JCM strain numbers (J), ISP strain numbers (I) and DDBJ DNA sequence ac-
region sequences are given along with the strain names. The IG and PC group symbols are shown
in bold letters. The bar labeled 0.05 indicates 5 base changes per 100 nucleotides.
Streptomyces lividans S. griseus [16],
[15],
S. coelicolor A3(2) S. ambofaciens [11] were
TK21 [14],
nucleotides in the stem were changed together. The
and
GCAT sequence in the loop was found to be highly
aligned. This enabled the selection of a 120-bp region
conserved, indicating that it may have an important
from nucleotide positions 158^277 of the 16S rRNA
role in the ribosome function. Only three strains,
S. ambofaciens,
gene of iable
K
as it includes the most var-
region [17].
To test the verity of a phylogenetic tree based on partial sequences of the 16S rRNA gene, we compared
two
phylogenetic
trees
constructed
by
alboniger (Fig. spheroides (not having
a
S. niveus
2),
(not
shown),
and
S. S.
shown), di¡ered from the others in
TCCT
sequence
at
the
corresponding
GCAT site.
the
Among the 89 strains, 57 kinds of 120-bp nucleo-
neighbor-joining method using published total and
tide sequences could be identi¢ed. In particular, 11
Streptomyces
identical sequences were shared by 47 of the strains :
strains [11,14^16,18]. We found the general topolo-
each sequence was shared by two to eight strains.
gies of the trees from the partial and total sequences
The groups containing these strains were designated
to be similar (Fig. 1), but the genetic distance to be
as `identity groups' (IGs). It is apparent from Fig. 3
more emphasized in the partial-sequence tree. This
that the strains in each IG belong to the same re-
observation indicated that the variation in the partial
spective numerical major cluster, the only exception
16S rDNA sequences covering the variable region is
being IG-G which includes strains from the major
su¤cient for deducing phylogenetic relationships of
clusters of
Streptomyces
fact
partial 16S rRNA sequences of seven
strains
at
the
intra-species
level,
that
S. exfoliatus
K
the
region
and is
S. violaceus.
the
most
From the
variable,
it
is
although these segments are probably too variable
thought that strains labeled as various di¡erent spe-
for comparison at the generic level.
cies names but sharing an identical sequence may actually belong to a single species even though minor
3.2. DNA sequences of 89 independent Streptomyces strains A 500-bp DNA sequence, partially encompassing the
16S
sample
rRNA
gene,
prepared
was
from
a
ampli¢ed
single
from
colony
of
a
DNA
each
in
K region was determined (see Fig. 3 for the
nucleotide
assisted
the
hyper-variable
characteristics
re-
To clarify the phylogenetic relationships of the 89
Streptomyces the variable
of
phenotypic
3.3. Phylogenetic relationship through the partial sequence
DDBJ accession numbers of these sequences). The sequences
their
sulted in their being classi¢ed as di¡erent.
of
the 89 strains, and the 120-bp sequence bearing the variable
di¡erences
region
strains, the 120-bp sequences bearing
K
region were subjected to computer-
phylogenetic
analysis
for
the
construction
from nucleotide positions 172^202 in 17 out of the
of a phylogenetic tree (Fig. 3). This tree has seven
89 strains, as well as some variations outside of the
major
region, are shown in Fig. 2. It has been suggested
PC-G), each comprised of four or more strains ; 60
that the hyper-variable region forms a stem and loop
of the 89 strains were classi¢ed into these seven clus-
structure in vivo in
S. ambofaciens
16S rRNA [11].
phylogenetic
clusters
(classi¢ed
as
PC-A
to
ters. Williams et al. [3] have shown that the numer-
S. albido£avus, S. anulatus, and S.
The conservation of the secondary structure is par-
ical major clusters,
ticularly notable, but the sequences forming the stem
halstedii,
are the most variable : the most of complementing
to form a large `super cluster'. This is partially in line
FEMSLE 7597 2-9-97
are closely related, and can be considered
M. Kataoka et al. / FEMS Microbiology Letters 151 (1997) 249^255
254
with our results, the exception being the strains of the
S. albido£avus major cluster ;
according to the
phylogenetic tree generated (Fig. 3), these are not closely related to the strains belonging to the major
S. anulatus, and S. halstedii. In our tree, strains of the S. albido£avus major cluster are
clusters of all the
grouped
into
phylogenetic
cluster
PC-D
with
less
than three base substitutions. The homogeneity of these strains has also been suggested by the results
of type cultures of
Streptomyces. IV. Species descriptions from
the second, third and fourth studies. Int. J. Syst. Bacteriol. 19, 391^512. [2] Shirling, E.B. and Gottlieb, D. (1972) Cooperative description of type strains of
Streptomyces.
V. Additional descriptions.
Int. J. Syst. Bacteriol. 22, 265^394. [3] Williams,
S.T.,
Goodfellow,
M.,
Alderson,
G.,
Wellington,
E.M.H., Sneath, P.H.A. and Sackin, M.J. (1983) Numerical classi¢cation of
Streptomyces
and related genera. J. Gen. Mi-
crobiol. 129, 1743^1813. [4] Williams, S.T., Goodfellow, M. and Alderson, G. (1989) Ge-
Streptomyces
AL .
from whole 16S rRNA sequences [19], chromosomal
nus
DNA hybridization [20], pyrolysis mass spectrometry
Bergey's Manual of Systematic Bacteriology, Vol. 4 (S.T. Wil-
[21] and fatty acid analysis [22]. PC-B is the largest cluster in our tree, comprising 19 of the 25 strains of the
S. anulatus major cluster and ¢ve of the seven S. halstedii major cluster but it is not
strains of the
closely related to PC-D. Strains of other numerical cluster
were
found
to
be
distributed among
other
phylogenetic clusters or were independent. The identity groups IG-J and IG-K are closely related to PCG. The two strains belonging to IG-K,
S. £aviscle-
rotiacus and S. minutisclerotiacus, were formerly classi¢ed as Chainia species, but were later transferred to Streptomyces [23].
Waksman
and
Henrici,
1943,
339
In :
liams, M.E. Sharpe and J.G. Holt, Eds.), pp. 2452^2492. Williams and Wilkins, Baltimore, MD. [5] Woese, C.R. (1987) Bacterial evolution. Microbiol. Rev. 51, 221^271. [6] Gladek, A., Mordarski, A., Goodfellow, M. and Williams, S.T. (1985) Ribosomal ribonucleic acid similarities in the classi¢cation of
Streptomyces.
FEMS Microbiol. Lett. 26, 175^
180. [7] Witt, D. and Stackebrandt, E. (1990) Uni¢cation of the gen-
Streptoverticillum and Streptomyces, and amendation of Streptomyces Waksman and Henrici 1943, 339AL . Syst. era
Appl. Microbiol. 13, 361^371. [8] Nakase, T. (1992) In : JCM Catalogue of Strains, 5th edn. (T. Nakase, Ed.), RIKEN, Saitama, Japan. [9] Higuchi,
R.G.
and
Ochman,
H.
(1989)
Production
of
In conclusion, we believe that the phylogenetic tree
single-stranded DNA templates by exonuclease digestion fol-
presented here will serve as a useful tool for rapid
lowing the polymerase chain reaction. Nucleic Acids Res. 17,
identi¢cation
of
newly isolated
the
phylogenetic
Streptomyces
localization
of
strains, and that it is
likely to prove more e¡ective than the conventional methods. Additionally, it should provide a means for
5865. [10] Saiki, R.K., Gelfand, D.H., Sto¡e, S., Scharf, S.J., Higuchi, R., Horn, G.T., Mullis, K.B. and Erlich, H.A. (1988) Primerdirected enzymatic ampli¢cation of DNA with a thermostable DNA polymerase. Science 239, 487^491.
easy and appropriate identi¢cation, which is espe-
[11] Pernodet, L.L., Boccard, F., Alegre, M.T., Gagnat, J. and
cially important in the fermentation industry in or-
è rineau, M. (1989) Organization and nucleotide sequence Gue
der to avoid taxonomic confusion of strains dealt with in patent literature.
analysis of a ribosomal RNA gene cluster from
ambofaciens.
Streptomyces
Gene 79, 33^46.
[12] Kimura, M. (1980) A simple method for estimating evolutionary rates of base substitutions through comparative studies of nucleotide sequences. J. Mol. Evol. 16, 111^120.
Acknowledgments We
are
[13] Saitou, N. and Nei, M. (1987) The neighbor-joining method : a
grateful
to
Tobias
Kieser
(John
Innes
new
method
for
16S
partially
Acids Res. 16, 370.
T.Y.
under
the
by
Grant-in
International
Aid
07044149
Scienti¢c
to
Research
Project of the Japanese Ministry of Science, Educa-
phylogenetic
trees.
Mol.
[14] Suzuki, Y. and Yamada, T. (1988) The nucleotide sequence of
Centre, UK) for helpful discussions. This work was supported
reconstructing
Biol. Evol. 4, 406^425.
rRNA gene from
Streptomyces lividans
TK21. Nucleic
[15] Baylis, H.A. and Bibb, M.J. (1989) The nucleotide sequence of a 16S rRNA gene from
Streptomyces coelicolor
A3(2). Nucleic
Acids Res. 18, 831.
tion, Sports and Culture.
[16] Kim, E., Kim, H., Kang, K.H., Kho, Y.H. and Park, Y.-H. (1991) Complete nucleotide sequence of a 16S ribosomal RNA
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