marY1, a Member of the gypsy Group of Long Terminal Repeat Retroelements from the Ectomycorrhizal Basidiomycete Tricholoma matsutake

doi:10.1128/AEM.66.8.3642-3645.2000

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Applied and Environmental Microbiology, August 2000, p. 3642-3645, Vol. 66, No. 8
0099-2240/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

marY1, a Member of the gypsy Group of Long Terminal Repeat Retroelements from the Ectomycorrhizal Basidiomycete Tricholoma matsutake

Hitoshi Murata¹^,^* and Akiyoshi Yamada²^,

Division of Bio-Resource Development, Forestry & Forest Products Research Institute, Tsukuba-Norin 305-8687,¹ and Department of Mushroom Science, Ibaraki Prefectural Forestry Center, Naka-machi, To 4692, Ibaraki 311-0122², Japan

Received 24 January 2000/Accepted 21 May 2000

	ABSTRACT

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We cloned an intact copy of a long terminal repeat retroelement designated marY1 from the ectomycorrhizal basidiomycete Tricholomamatsutake. The reverse transcriptase domain is found in T. matsutakeand Tricholoma magnivelare worldwide. This finding suggests thatretroelements associate with ectomycorrhizal basidiomycetes andmay be useful as genetic markers for identification, phylogeneticanalysis, and mutagenesis of this fungalgroup.

	TEXT

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Retroelements are retrovirus-like DNA elements found in eukaryotic genomes (3, 4, 16) which may replicate throughan RNA intermediate and are often found at multiple dispersedlocations within the genome (2, 3, 4, 13, 15, 16).Retroelements have been recognized in some ascomycetes as geneticmarkers (1, 6, 7, 14, 17).

Matsutake and American matsutake are economically important edible mushrooms produced by the ectomycorrhizal basidiomycetesTricholoma matsutake and Tricholoma magnivelare, respectively(12). They form mycorrhizae with some Pinaceae plants (12).We previously identified a 967-bp sequence encoding part of aretroelement polyprotein in the genome of T. matsutake strainY1 and subsequently found the RNase H domain in T. matsutake andT. magnivelare (18). Our objective in this study was to isolateand characterize a full-length copy of this retroelement fromT. matsutake. This retroelement will be used to develop new meansof identification, phylogenetic analysis, and mutagenesis of ectomycorrhizalbasidiomycetes.

Cloning of a full-length copy of the retroelement. A genomic library of T. matsutake strain Y1 constructed in $lambda$ EMBL3 (Stratagene, La Jolla, Calif.) was probed with a 550-bpBamHI-XbaI fragment from the 967-bp multiple-copy sequence previouslycloned in plasmid pHHM145 (Fig. 1) (18, 21). The probe DNAwas labeled with [ $alpha$ -³²P]dCTP by the random primer extension (New England Nuclear, Boston,Mass.). Of approximately 3,000 plaques, 14 hybridized with theprobe. DNA was isolated from all the positive $lambda$ EMBL3 clones, digestedwith restriction endonucleases, transferred to a nylon membrane,and hybridized with the [ $alpha$ -³²P]dCTP-labeled 550-bp BamHI-XbaI fragment (18, 21). Southernhybridizations identified a clone, $lambda$ A2, which contains the homologuein 2.8-kb BamHI, 9.2-kb EcoRI, and 8.5-kb KpnI fragments whosesizes correspond to those previously identified in genomic Southernhybridizations with strains of T. matsutake (18). Therefore,we hypothesized that $lambda$ A2 contained a full-length copy of the retroelement.

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FIG. 1. Characteristics of marY1 cloned into $lambda$ A2. Insert DNA is represented by a solid black line. The thin line represents adjacent $lambda$ EMBL3 vector DNA. Restriction sites of BamHI (B), BglII (G), EcoRI (E), HindIII (H), KpnI (K), SalI (S), and XhoI (X) are given. The arrow denotes the direction of marY1 and the location of the fragment previously cloned in pHHM145 (18). The solid black bar and the hatched bar underneath the insert DNA indicate probes for the plaque hybridizations used to identify $lambda$ A2 and Southern hybridizations to determine the distribution of the marY1 homologues in fungal strains, respectively. Domains corresponding to 5' LTR, 3' LTR, gag, prt, and pol are given. The location of a putative ribosomal frameshifting site is indicated by the arrowhead. A zinc-finger DNA-binding site in the gag gene product, a consensus catalytic site in prt, and domains of reverse transcriptase (RT), RNase H (RH), and integrase (IT) are aligned at the bottom.

The 8.5-kb KpnI fragment from $lambda$ A2 contains the 2.8-kb BamHI fragment homologous to the 967-bp multiple-copy sequence and islarge enough to encode a retroelement of 5 to 8 kb. The KpnI fragmentwas digested with BglII to generate 5.5-kb and 3.0-kb KpnI-BglIIfragments to increase the ligation efficiency and to orient thefragment in the vector. These fragments were ligated into theKpnI-BamHI site of pBluescript SK+ (Stratagene, La Jolla, Calif.),generating plasmids pHHM147 and pHHM148,respectively.

Identification of the LTR retroelement marY1. The inserts of pHHM147 and pHHM148 were sequenced with an ABI prism 377 autosequencer (Perkin-Elmer Japan, Urayasu, Japan).Data were analyzed using the computer software GENETIX-Mac ver.9.0 (Software Development Co., Tokyo, Japan), Clustal W (23),and Advanced BLAST Search provided by the National Center forBiotechnology Information (http://www.ncbi.nlm.nih.gov /BLAST).Unless stated otherwise, the position of a sequence is expressedas the number of base pairs from the 5' end of marY1 (marY1 =a retroelement of T. matsutake strain Y1 [see below]).

The 6,046-bp element carries identical 425-bp long terminal direct repeats (LTRs) (Fig. 1). The LTRs contain the terminalsequences of 5'-TG...TA-3' instead of 5'-TG...CA-3', which are presentin the LTRs of many, but not all, retroelements (3, 4).The LTR also has several conserved sequences, including a 5-bpdirect repeat of ATGTT immediately outside the 5' and the 3' LTRs.This apparent target site duplication is a typical feature generatedduring the retrotransposon integration process (13, 16). Inaddition, the AT-rich target site duplication associated withmarY1 is consistent with those reported for many retrotransposoninsertion sites in other organisms (3, 16).

The 5' LTR of marY1 has three CT-rich sequences, i.e., a 33-bp stretch starting at bp 77, a 25-bp stretch at bp 231, and a43-bp stretch at bp 318. The third CT-rich sequence may correspondto the ct box immediately upstream of the transcription initiationsite in the Aspergillus nidulans gpdA gene promoter (20). Thisconclusion is based on the position of the third CT-rich sequencerelative to that of the TTCCA sequence at bp 104, which is identicalto the enhancer of Ty1 of Saccharomyces cerevisiae (25) andthe qa-2 gene of Neurospora crassa (9). Like the ct box ofA. nidulans gpdA (20), the third CT-rich sequence of marY1 associateswith a stretch of direct repeat. The occurrence of CT-rich sequencein the 5' LTR was also reported in Grasshopper, an LTR retroelementof Magnaporthe grisea (6). Upstream and downstream of the TTCCAsequence, we identified a sequence similar to a CCAAT-like transcriptionactivation signal and two putative TATA domains (4, 24).A GC-rich sequence upstream of the putative CCAAT-like signalis similar to the GC-rich box required for DNA binding by sometranscription factors (24). We did not identify a potentialtRNA primer binding site for minus-strand DNA synthesis, whichis generally located immediately after the 3' end of the 5' LTR,but we did find a 13-bp purine-rich sequence, which could be theprimer binding site for plus-strand DNA synthesis, immediatelyupstream of the 5' end of the 3' LTR (3, 24).

Characterization of ORFs in marY1. Three open reading frames (ORFs) occur on the same strand in the same direction in marY1 (Fig. 1). The first ORF begins atthe ATG codon at bp 592 to 594 and continues to a TGA stop codonat bp 1708 to 1710 (Fig. 1). This ORF is predicted to encode aprotein with 352 amino acids that is 41 and 39% similar to theamino acid sequences of the putative gag gene products of skippy,which is a retroelement of Fusarium oxysporum, and MAGGY of M.grisea, respectively (1, 7). The putative protein of marY1also was similar to the gag gene products of a number of otherretrotransposons and retroviruses. This protein should have azinc-finger DNA-binding domain (C-X2-C-X9-C) at amino acid positions304 to 321 (5). The amino acid sequence of the putative zinc-fingerDNA-binding domain encoded in marY1 is 78% similar to that ofovine pulmonary carcinoma virus (10). The molecular mass ispredicted to be 42 kDa, which is smaller than most gag gene products,i.e., 60 to 80 kDa (24). However, a putative ribosomal frameshiftsite occurs at the 3' end of gag (Fig. 1). If the TGA at bp 1708to 1710 is bypassed by a ribosomal frameshift at bp 1691 to 1692,then the predicted molecular mass is 63.6 kDa and it would bea gag-prt fusion. Such polyproteins are known in some retroviruses,such as human immunodeficiency virus, mouse mammary tumor virus,and human T-cell leukemia virus (24).

A second ORF extends from an ATG start codon at bp 1962 to 1964 to a TGA stop codon at bp 2292 to 2294 (Fig. 1). This ORFis predicted to encode a peptide of 111 amino acid residues witha molecular mass of 12.2 kDa. It is similar in size to the acidprotease of retroviruses (24) and has a conserved catalyticsite that is similar to those of other acid proteases (24).The amino acid sequence of a putative acid protease encoded inmarY1 is 52 and 49% similar to those of skippy and MAGGY, respectively(1, 7).

The third ORF begins at the ATG codon at bp 2436, ends at the TAG codon at bp 5609, and is predicted to encode a protein productof 1,057 amino acid residues with a molecular mass of 122.2 kDa(Fig. 1). The putative amino acid sequence is similar to thoseof the pol gene products of a number of retroviruses and retrotransposonsand is particularly similar to the putative reverse transcriptase,RNase H, and integrase domains of MAGGY of M. grisea (59% similarity),skippy of F. oxysporum (54% similarity), and CfT-I of Cladosporiumfulvum (54% similarity) (1, 7, 17). Of those, the domainV of reverse transcriptase in marY1 is most conserved, and hasa perfect match with the YXDD sequence (where X is unknown) ofthe proposed reverse transcriptase active site (24).

In general, LTR retroelements are classified into two groups (3, 4, 15). Those in the gypsy group have two or threeORFs, the first encoding gag, the second pol, and the third env,and are regarded as a group closely related to retroviruses (3,13, 15). Although pol generally encodes the protease gene(prt) in retrotransposons (3, 4, 13, 15), prt in someretroviruses occurs as the second ORF prior to the ORF of pol(24). These ORFs are transcribed into a polycistronic mRNA andtranslated into several polyproteins, which often require ribosomalframeshifting, nonsense suppression, and/or splicing to bypassstop codons located between the ORFs, especially the one associatedwith the 3' end of gag (13, 24). The pol gene in gypsy elementsgenerally encodes domains in the following order: prt-reversetranscriptase-RNase H-integrase (2, 3, 15). The othergroup of LTR retroelements is the copia group, which featuresa single ORF encoding domains in the following order: gag-prt-integrase-reversetranscriptase-RNase H (2, 3, 15). While a significantnumber of copia-type retroelements are recognized in many plantspecies (2, 11, 15), all LTR retroelements identified sofar in plant-infecting fungi belong to the gypsy group (1,6, 7, 17). marY1, the first reported retroelement in anectomycorrhizal basidiomycete, also belongs to the gypsy groupof LTRretroelements.

Conservation of marY1 in the genome of T. matsutake. To determine whether marY1 is ubiquitous in T. matsutake and T. magnivelare, we hybridized the [ $alpha$ -³²P]dCTP-labeled 1.1-kb SalI-BamHI fragment, which contains thereverse transcriptase domain (Fig. 1), to genomic digests of 18T. matsutake strains and two T. magnivelare strains from Canada(Fig. 2) (18). Hybridization was detected in all 20 strains(Fig. 2). A reverse transcriptase domain was found on a 1.2-kbBamHI fragment in T. matsutake and on a 5.7-kb BamHI fragmentin T. magnivelare (Fig. 2). In addition, two larger BamHI fragmentsthat hybridized weakly with the probe also were present in allsamples of T. matsutake (Fig. 2). The length of the EcoRI fragmentcarrying the homologue of the probe, however, was apparently conservedin both T. matsutake and T. magnivelare (Fig. 2).

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FIG. 2. Southern hybridization analysis of genomic digests of T. matsutake and T. magnivelare probed with the reverse transcriptase domain of marY1. (A) BamHI digests. (B) EcoRI digests. Lanes 1 to 18, T. matsutake (18): lane 1, Y1 (from Ibaraki, eastern Honshu, the main island of Japan); lane 2, Y59 (from Yamaguchi, far western Honshu); lane 3, OK-T4 (from Okayama, western Honshu); lane 4, MR32 (from Hyogo, western Honshu); lane 5, TM-8 (from Kyoto, western Honshu); lane 6, TM15 (from Iwate, northern Honshu); lane 7, Tm-H507 (from Hiroshima, far western Honshu); lane 8, TMT4 (from Tokushima, Shikoku island of Japan); lane 9, Tm31 (from Kyongsang North, Republic of Korea); lane 10, K1 (from the Republic of Korea through a retailer); lane 11, NK1 (from Democratic People's Republic of Korea through a retailer); lane 12, TM-9 (from People's Republic of China through a retailer); lane 13, CHI1 (from People's Republic of China through a retailer); lane 14, BH1 (from Kingdom of Bhutan through a retailer); lane 15, TM-5 (from Kingdom of Morocco through a retailer); lane 16, MC1 (from Kingdom of Morocco through a retailer); lane 17, TM-4 (from Mexico through a retailer); lane 18, MX1 (from Mexico through a retailer). Lanes 19 to 20, T. magnivelare (18): lane 19, CA1 (from Canada through a retailer); lane 20, Tp-C3 (from Canada through a retailer). Molecular markers (kb) are indicated at the left.

We also attempted to hybridize the probe carrying the 1.1-kb SalI-BamHI fragment to genomic digests of Suillus bovinus strainMR16 (18) and Rhizopogon rubescens strain MR11 (18), fungalspecies that have been well characterized in terms of ectomycorrhizalsymbiosis in Pinus sp. plants (22). However, we could not detectany homologues of a reverse transcriptase domain encoded in marY1.

Retroelements have been recognized in a wide range of eukaryotes and, in some cases, used as genetic markers to investigatephylogeny, to generate mutants and recombinants, and to identifymutated genes (2, 3, 4, 8, 11, 15, 16, 19).In ectomycorrhizal basidiomycetes, however, retroelements hadnot been previously described. The discovery of a full-lengthcopy of a retroelement in T. matsutake suggests that ectomycorrhizalfungi also carry retroelements, some of which could function astransposons to induce mutants or used as genetic markers for phylogeneticanalysis and identification of ectomycorrhizae. The nucleotideand putative amino acid sequences of marY1 will serve as a referencein the search for retroelements in other ectomycorrhizalbasidiomycetes.

The genetic manipulation of marY1 could lead to the development of a transposon-mediated analysis system in ectomycorrhizalfungi, since marY1 is apparently intact and might be mobile giventhe correct stimulus. Transposon-mediated analysis is effectiveif the organism to be subjected to mutagenesis does not carryany copies of the transposon that is to be introduced (11, 15,16). In this respect, it is very important that S. bovinus andR. rubescens do not have marY1, and this element might be usedfor introducing mutations into these ectomycorrhizal symbionts.We are currently investigating whether marY1 functions in heterologousfungal cells and expect to utilize marY1 to further transposon-mediatedresearch with ectomycorrhizalfungi.

Nucleotide sequence accession number. The nucleotide sequence of the marY1 retroelement has been deposited in the GenBank, EMBL, and DDBJ databases under the accessionnumber AB028236.

	ACKNOWLEDGMENTS

This work was supported by the Biotechnology in Ectomycorrhizae Program of the Ministry of Agriculture, Forestry and FisheriesofJapan.

The authors thank forest experiment stations located in the following prefectures in Japan for the supply of fungal strains:Chiba, Fukui, Hiroshima, Hyogo, Iwate, Kyoto, Okayama, Shiga,Tokushima, andYamaguchi.

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Bio-Resource Development, Forestry & Forest Products Research Institute,P.O. Box 16, Tsukuba-Norin, 305-8687, Japan. Phone: 81-298-73-3211.Fax: 81-298-73-3795. E-mail: murmur{at}ffpri.affrc.go.jp.

Present address: Shinshu University, Minami Minowa 8304, Nagano, 399-4598,Japan.

REFERENCES

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7. Farman, M. L., Y. Tosa, N. Nitta, and S. A. Leong. 1996. MAGGY, a retrotransposon in the genome of the rice blast fungus Magnaporthe grisea. Mol. Gen. Genet. 251:665-674[Medline].

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10. Hecht, S. J., J. O. Carlson, and J. C. DeMartin. 1994. Analysis of a type D retroviral capsid gene expressed in ovine pulmonary carcinoma and present in both affected and unaffected sheep genomes. Virology 202:480-484[CrossRef][Medline].

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12. Hosford, D., D. Pilz, R. Molina, and M. Amaranthus. 1997. Ecology and management of the commercially harvested American matsutake mushroom, p. 1-68. In U.S. Department of Agriculture Forest Service Pacific Northwest Research Station General Technical Report PNW-GTR-412. U.S. Department of Agriculture, Washington, D.C.

13. Hutchison, C. A., III, S. C. Hardies, D. D. Loeb, W. Ronald Shehee, and M. H. Edgell. 1989. LINEs and related retroposons: long interspersed repeated sequences in the eukaryotic genome, p. 593-617. In D. E. Berg, and M. M. Howe (ed.), Mobile DNA. American Society for Microbiology, Washington, D.C.

14. Kinsey, J. A., and J. Helber. 1989. Isolation of a transposable element from Neurospora crassa. Proc. Natl. Acad. Sci. USA 86:1929-1933[Abstract/Free Full Text].

15. Kumar, A. 1996. The adventures of the Ty1-copia group of retrotransposons in plants. Trends Genet. 12:41-43[CrossRef][Medline].

16. Lucas, H., F. Feuerbach, K. Kunert, M.-A. Grandbastien, and M. Caboche. 1995. RNA-mediated transposition of the tobacco retrotransposon Tnt1 in Arabidopsis thaliana. EMBO J. 14:2364-2373[Medline].

17. McHale, M. T., I. N. Roberts, S. M. Noble, C. Beaumont, M. P. Whitehead, D. Seth, and R. P. Oliver. 1992. CfT-I: an LTR-retrotransposon in Cladosporium fulvum, a fungal pathogen of tomato. Mol. Gen. Genet. 233:337-347[Medline].

18. Murata, H., A. Yamada, and K. Babasaki. 1999. Identification of repetitive sequences containing motifs of retrotransposons in the ectomycorrhizal basidiomycete Tricholoma matsutake. Mycologia 91:766-775[CrossRef].

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1.	Anaya, N., and M. I. G. Roncero. 1995. skippy, a retrotransposon from the fungal plant pathogen Fusarium oxysporum. Mol. Gen. Genet. 249:637-647[CrossRef][Medline].
2.	Bennetzen, J. L. 2000. Transposable element contributions to plant gene and genome evolution. Plant Mol. Biol. 42:251-269[CrossRef][Medline].
3.	Bingham, P. M., and Z. Zachar. 1989. Retrotransposons and the FB transposon from Drosophila melanogaster, p. 485-502. In D. E. Berg, and M. M. Howe (ed.), Mobile DNA. American Society for Microbiology, Washington, D.C.
4.	Boeke, J. D. 1989. Transposable elements in Saccharomyces cerevisiae, p. 335-374. In D. E. Berg, and M. M. Howe (ed.), Mobile DNA. American Society for Microbiology, Washington, D.C.
5.	Covey, S. N. 1986. Amino acid sequence homology in gag region of reverse transcribing elements and the coat protein gene of cauliflower mosaic virus. Nucleic Acids Res. 14:623-633[Abstract/Free Full Text].
6.	Dobinson, K. F., R. E. Harris, and J. E. Hamer. 1993. Grasshopper, a long terminal repeat (LTR) retroelement in the phytopathogenic fungus Magnaporthe grisea. Mol. Plant-Microbe Interact. 6:114-126[Medline].
7.	Farman, M. L., Y. Tosa, N. Nitta, and S. A. Leong. 1996. MAGGY, a retrotransposon in the genome of the rice blast fungus Magnaporthe grisea. Mol. Gen. Genet. 251:665-674[Medline].
8.	Flavell, A. J., and D. B. Smith. 1992. A Ty1-copia group retrotransposon sequence in a vertebrate. Mol. Gen. Genet. 233:322-326[CrossRef][Medline].
9.	Geever, R. F., M. E. Case, B. M. Tyler, F. Buxton, and N. H. Giles. 1983. Point mutations and DNA rearrangements 5' to the inducible qa-2 gene of Neurospora allow activator protein-independent transcription. Proc. Natl. Acad. Sci. USA 80:7298-7302[Abstract/Free Full Text].
10.	Hecht, S. J., J. O. Carlson, and J. C. DeMartin. 1994. Analysis of a type D retroviral capsid gene expressed in ovine pulmonary carcinoma and present in both affected and unaffected sheep genomes. Virology 202:480-484[CrossRef][Medline].
11.	Hirochika, H. 1997. Retrotransposons of rice: their regulation and use for genome analysis. Plant Mol. Biol. 35:231-240[CrossRef][Medline].
12.	Hosford, D., D. Pilz, R. Molina, and M. Amaranthus. 1997. Ecology and management of the commercially harvested American matsutake mushroom, p. 1-68. In U.S. Department of Agriculture Forest Service Pacific Northwest Research Station General Technical Report PNW-GTR-412. U.S. Department of Agriculture, Washington, D.C.
13.	Hutchison, C. A., III, S. C. Hardies, D. D. Loeb, W. Ronald Shehee, and M. H. Edgell. 1989. LINEs and related retroposons: long interspersed repeated sequences in the eukaryotic genome, p. 593-617. In D. E. Berg, and M. M. Howe (ed.), Mobile DNA. American Society for Microbiology, Washington, D.C.
14.	Kinsey, J. A., and J. Helber. 1989. Isolation of a transposable element from Neurospora crassa. Proc. Natl. Acad. Sci. USA 86:1929-1933[Abstract/Free Full Text].
15.	Kumar, A. 1996. The adventures of the Ty1-copia group of retrotransposons in plants. Trends Genet. 12:41-43[CrossRef][Medline].
16.	Lucas, H., F. Feuerbach, K. Kunert, M.-A. Grandbastien, and M. Caboche. 1995. RNA-mediated transposition of the tobacco retrotransposon Tnt1 in Arabidopsis thaliana. EMBO J. 14:2364-2373[Medline].
17.	McHale, M. T., I. N. Roberts, S. M. Noble, C. Beaumont, M. P. Whitehead, D. Seth, and R. P. Oliver. 1992. CfT-I: an LTR-retrotransposon in Cladosporium fulvum, a fungal pathogen of tomato. Mol. Gen. Genet. 233:337-347[Medline].
18.	Murata, H., A. Yamada, and K. Babasaki. 1999. Identification of repetitive sequences containing motifs of retrotransposons in the ectomycorrhizal basidiomycete Tricholoma matsutake. Mycologia 91:766-775[CrossRef].
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