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Co-localization of Trax and Mea2 in Golgi Complex of Pachytene Spermatocytes in the Mouse

Miyuki Matsuda, Masaaki Kondo, Shin-ichi Kashiwabara, Mitsuyo Yoshihara, Shizuyo Sutou and Shoichi Matsukuma

Kanagawa Cancer Center Research Institute, Yokohama (MM,MY,SM); Ito Life Sciences Inc., Ibaraki (MK); Institute of Applied Biochemistry, University of Tsukuba, Tsukuba (SK); and School of Pharmacy, Shujitsu University (SS), Okayama, Japan

Correspondence to: Shoichi Matsukuma, PhD, Kanagawa Cancer Center Research Institute, Nakao 1-1-2, Asahi-ku, Yokohama 241-0815, Japan. E-mail: matsukum{at}gancen.asahi.yokohama.jp

	Summary

Top Summary Literature Cited

 
A golgin family protein, Mea2, is expressed at enhanced level in pachytene spermatocytes and is indispensable for mouse spermatogenesis. Because Trax was shown to interact with Mea2 in yeast two-hybrid, we investigated the localization of Trax in pachytene spermatocytes with immunofluorescent staining. Trax was found to accumulate in the Golgi complex of mid-late pachytene spermatocytes and intermingled with granular Mea2 signal in the central region. In a subline of the Mea2 mutant mouse, a truncated form of Mea2 devoid of the N-terminal region, Mea2, was expressed. It localized to the rim of Golgi complex and thus occupied a region separate from that of Trax.

(J Histochem Cytochem 52:1245–1248, 2004)

Key Words: Golgi complex • spermatocytes • mutant mouse • golgin-160

THE GOLGI COMPLEX in pachytene spermatocytes is well developed but its function is not understood. A Golgi protein, Mea2, is expressed at enhanced level in spermatocytes (Banu et al. 2002) and its disruption at a transgene insertion resulted in sterility in the homozygous mutant male mice (Matsukuma et al. 1999). The homozygous mutant males expressed a truncated form of Mea2, Mea2, at variable levels in mid-late pachytene spermatocytes. It was shown that a certain level of Mea2 expression was necessary for viability of late pachytene spermatocytes (Banu et al. 2002).

Mea2H was a subline of T604 transgenic mouse derived from the proband of a fertile male homozygote. Unlike the original mouse line in which only 9% of homozygous males showed fertility, the reproductive capability of Mea2H males was improved significantly and they sired consistently at ages above 10 weeks. However, testis weight remained at 49% of the hemizygous males, and the epididymal sperm count in Mea2H remained at 29% of the hemizygotes on average (Table 1). Sperm production of Mea2H homozygous males exhibited variation from 3.5 x 10⁵ to 2 x 10⁷ inclusive of apparently exceptional infertile animals. On the other hand, sperm production of the homozygotes in the original line was below 3.5 x 10⁵ in 61% of individuals.

A full-length cDNA fragment of mouse Trax was produced by PCR with primers (5'-GGATCCATGAACGGCAAAGAAGGACCA-3', 5'-CCAGGAGCTCCTTAGAGAGCA-3') and the template of Trax cDNA plasmid clone (pI151). The fragment was used to create a GST–Trax fusion protein in pGEX-6P-1. The recombinant fusion protein bound to glutathione Sepharose beads (GS4B) was washed and treated with PreScission protease (Amersham Bioscience; Piscataway, NJ) at 4C overnight. The cleaved mixture was separated with 12% SDS-PAGE. Trax (33 kD) was recovered as a gel strip cut out according to colored size markers. The cut-out gel was homogenized with an equal volume of PBS and was used to immunize guinea pigs by injecting 75 µg of Trax protein with Freund's complete adjuvant every 2 weeks over a period of 12 weeks.

The recombinant Trax recovered from the SDS-PAGE gel strip described above was electro-eluted (Electro-Eluter model 422; Bio-Rad Laboratories, Hercules, CA) and coupled to actigel ALD (Sterogene Bioseparations; Carlsbad, CA) for affinity-purification of anti-Trax antibody. The antibody eluted with ActiSep elution medium (Sterogene Bioseparations) was stored at 4C in PBS containing 0.02% sodium azide.

With the affinity-purified anti-Trax antibody, a major band at 33 kD of the size of mouse Trax and a minor band at 25 kD were detected in the immunoblot of normal mouse testis tissue lysate (Figure 1A) . A DDY mouse (SLC; Shizuoka, Japan) was used for fractionation of testicular cells (Bellvé 1993). When the fractions of pachytene spermatocytes, round spermatids, and elongated spermatids were examined in the immunoblot, the minor band was greatly reduced in pachytene spermatocytes (at 80% purity) in contrast to the gradual increase of the minor band in round and elongated spermatids (Figure 1B). In pachytene spermatocytes, 33-kD Trax protein alone seemed to be present and detected by the antibody.

View larger version (41K): [in this window] [in a new window]   Figure 1 Specificity of anti-Trax antibody in testis tissue. (A) Immunoblot of the whole testis tissue lysate (W) of normal adult mice was immunoreacted with anti-Trax antibody (right) and compared with unreacted control (left). (B) Immunoblot of whole testis (W), and the fractionated germ cells of pachytene spermatocytes (P), round spermatids (R), and elongated spermatids (E) was detected with anti-Trax antibody. Trax at 33 kD is indicated by a black arrowhead and a smaller band at 25 kD by a gray arrowhead.

Testis of an 18-day-old mouse was enriched with mid-late pachytene spermatocytes, mostly devoid of spermatids, and thus provided a suitable material for examining localization of Trax with immunostaining. In C3H pachytene spermatocytes, Trax was accumulated in the central region of an enlarged Golgi complex where Mea2 was detected intermingled with Trax (Figures 2A–2C) . GM130 was detected in the rim region of the Golgi complex in separation from Mea2 (Figures 2Dand 2E). In pachytene spermatocytes of Mea2H homozygotes, Trax was observed to accumulate in the central region of the Golgi complex (Figure 2F) as in C3H. Mea2, on the other hand, was localized not in the central region but in the rim domain where GM130 was present (Figures 2G–2J).

View larger version (56K): [in this window] [in a new window]   Figure 2 Immunofluorescent detection of Trax, Mea2, and Mea2 in Golgi complex of mid-late spermatocytes of prepubertal and adult mice. Wildtype (A–E) and Mea2H homozygous (F–J) testes of 18-day-old mice were immunostained with three layers of anti-Trax (A,F), anti-Mea2 (B,G), and anti-GM130 (D,I) antibodies and detected with the secondary antibodies. The merged views of pseudocolor images for Trax and Mea2 (C), Mea2 and GM130 (E), Trax and Mea2 (H), and Mea2 and GM130 (J) for the field corresponding to the rectangles in A and F are shown. Arrows in C and H indicate nuclei. Enlarged views are shown for the Golgi complexes of mid-late pachytene spermatocytes of wild-type (K,L) and Mea2H homozygous (N,O) adult testes immunostained with two layers of anti-Trax (K,N) and anti-Mea2 (L,O) antibodies followed by the secondary antibodies conjugated with separate fluorochromes. Merged views for Trax and Mea2 (M) and for Trax and Mea2 (P) are shown. Bars = 5 µm.

The co-existence of Trax and Mea2 in the central region of Golgi complex in wild-type mid-late pachytene spermatocytes implied that the molecular interaction between the two molecules could occur in the organelle. On the other hand, Trax and Mea2, apparently localized in separate regions of the Golgi complex, might be restricted from interaction. Because spermatogenesis in Mea2H mice was significantly restored, the restricted interaction between Mea2 and Trax in the Golgi complex seemed to have little influence on the survival of mutant spermatocytes and their differentiation to fertile sperm. However, considering that the spermatogenic potency in Mea2H mice was still partial, the possibility remained that the molecular interaction between Mea2 and Trax could be important for augmentation of reproductive potency through unknown mechanisms.

The NLS motif in Trax (Aoki et al. 1997) was presumably important for the nuclear transport of Trax. We actually recognized Trax signal in some nuclei of late pachytene spermatocytes (Figures 2C and 2H). The significance of the transient shift of subcellular localization from cytoplasm to Golgi complex and to nucleus in pachytene spermatocytes remains unknown.

Mea2 consists of N-terminal proline-rich and serine-rich domains and coiled-coil regions (Misumi et al. 1997). Our results implied that the N-terminal region, lost in Mea2, might contain a motif important for localization of Mea2 in the central region of the Golgi complex in mid-late pachytene spermatocytes. A small Golgi protein, GCP16, was recently shown to interact with the human orthologue of Mea2, GCP170/golgin-160, in the N-terminal region (Ohta et al. 2003) and could be a candidate protein to regulate localization of Mea2 within the Golgi complex.

	Acknowledgments

 
Supported in part by a grant from Ministry of Health, Labor and Welfare, Japan. The animal experiment code of Kanagawa Cancer Center was observed.

	Footnotes

 
Received for publication March 2, 2004; accepted April 12, 2004

	Literature Cited

Top Summary Literature Cited

 

Aoki K, Ishida R, Kasai M (1997) Isolation and characterization of a cDNA encoding a translin-like protein, TRAX. FEBS Lett 401:109–112[CrossRef][Medline]

Banu Y, Matsuda M, Yoshihara M, Kondo M, Sutou S, Matsukuma S (2002) A Golgi matrix protein gene, Golga3/Mea2, rearranged and re-expressed in pachytene spermatocytes restores spermatogenesis in the mouse. Mol Reprod Dev 61:288–301[CrossRef][Medline]

Bellvé A (1993) Purification, culture, and fractionation of spermatogenic cells. Methods Enzymol 225:84–113[Medline]

Bray J, Chennathukuzhi V, Hecht N (2002) Identification and characterization of cDNAs encoding four novel proteins that interact with translin associated factor-X. Genomics 79:799–808[CrossRef][Medline]

Matsukuma S, Kondo M, Yoshihara M, Matsuda M, Utakoji T, Sutou S (1999) Mea2/Golga3 gene is disrupted in a line of transgenic mice with a reciprocal translocation between chromosomes 5 and 19 and is responsible for a defective spermatogenesis in homozygotes. Mamm Genome 10:1–5[CrossRef][Medline]

Misumi Y, Sohda M, Yano A, Fujiwara T, Ikehara Y (1997) Molecular characterization of GCP170, a 170-kDa protein associated with the cytoplasmic face of the Golgi membrane. J Biol Chem 272:23851–23858[Abstract/Free Full Text]

Nakamura N, Rabouille C, Watson R, Nilsson T, Hui N, Slusarewicz P, Kreis TE, et al. (1995) Characterization of a cis-Golgi matrix protein, GM130. J Cell Biol 131:1715–1726[Abstract/Free Full Text]

Ohta E, Misumi Y, Sohda M, Fujiwara T, Yano A, Ikehara Y (2003) Identification and characterization of GCP16, a novel acylated Golgi protein that interacts with GCP170. J Biol Chem 278:51957–51967[Abstract/Free Full Text]

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This Article Abstract Full Text (PDF) Alert me when this article is cited Alert me if a correction is posted Services Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via Google Scholar Google Scholar Articles by Matsuda, M. Articles by Matsukuma, S. Search for Related Content PubMed PubMed Citation Articles by Matsuda, M. Articles by Matsukuma, S. Social Bookmarking                      What's this?

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