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Development of rat tetraploid and chimeric embryos aggregated with diploid cells

Published online by Cambridge University Press:  01 November 2006

T. Shinozawa ,
A. Sugawara ,
A. Matsumoto ,
Y-J. Han ,
I. Tomioka ,
K. Inai ,
H. Sasada ,
E. Kobayashi ,
H. Matsumoto  and
E. Sato
T. Shinozawa
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
A. Sugawara
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
A. Matsumoto
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
Y-J. Han
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
I. Tomioka
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
K. Inai
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
H. Sasada
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
E. Kobayashi
Affiliation:
Division of Organ Replacement Research, Center for Molecular Medicine, Jichi Medical School, Tochigi, Japan.
H. Matsumoto*
Affiliation:
Laboratory of Animal Breeding and Reproduction, Faculty of Agriculture, Utsunomiya University, Utsunomiya, Tochigi, Japan.
E. Sato
Affiliation:
Laboratory of Animal Reproduction, Graduate School of Agricultural Science, Tohoku University, Sendai, Japan.
*
All correspondence to: H Matsumoto. Laboratory of Breeding and Reproduction, Division of Animal Science, Department of Bioproductive Science, Faculty of Agriculture, Utsunomiya University, 350 Mine-machi, Utsunomiya, Tochigi 321-8505, Japan. Tel: +81 28649 5432. Fax: +81 28649 5431. e-mail: matsu@cc.utsunomiya-u.ac.jp
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Summary

In the present study, we examined the preimplantation and postimplantation development of rat tetraploid embryos produced by electrofusion of 2-cell-stage embryos. Developmental rate of tetraploid embryos to morula or blastocyst stage was 93% (56/60) and similar to that found in diploid embryos (95%, 55/58). After embryo transfer, rat tetraploid embryos showed implantation and survived until day 8 of pregnancy, however the conceptuses were aberrant on day 9. In mouse, tetraploid embryos have the ability to support the development of blastomeres that cannot develop independently. As shown in the present study, a pair of diploid blastomeres from the rat 8-cell-stage embryo degenerated immediately after implantation. Therefore, we examined whether rat tetraploid embryos have the ability to support the development of 2/8 blastomeres. We produced chimeric rat embryos in which a pair of diploid blastomeres from an 8-cell-stage green fluorescent protein negative (GFP−) embryo was aggregated with three tetraploid blastomeres from 4-cell GFP-positive (GFP+) embryos. The developmental rate of rat 2n(GFP−) ↔ 4n(GFP+) embryos to the morula or blastocyst stages was 93% (109/117) and was similar to that found for 2n(GFP−) ↔ 2n(GFP+) embryos (100%, 51/51). After embryo transfer, 2n(GFP−) ↔ 4n(GFP+) conceptuses were examined on day 14 of pregnancy, the developmental rate to fetus was quite low (4%, 4/109) and they were all aberrant and smaller than 2n(GFP−) ↔ 2n(GFP+) conceptuses, whereas immunohistochemical analysis showed no staining for GFP in fetuses. Our results suggest that rat tetraploid embryos are able to prolong the development of diploid blastomeres that cannot develop independently, although postimplantation development was incomplete.

Keywords

EmbryoPreimplantation developmentPostimplantation developmentRatTetraploid
Type
Research Article
Information
Zygote , Volume 14 , Issue 4 , November 2006 , pp. 287 - 297
Copyright
Copyright © Cambridge University Press 2006

Introduction

Tetraploid mouse embryos are produced either by the inhibition of cleavage at an early stage or by fusion of blastomeres. Inhibition of cleavage, in order to cause duplication of the genome without cell division, has been accomplished using inhibitors of cytokinesis, such as colchicines (Edwards, Reference Edwards1958) and cytochalasin B (Snow, Reference Snow1973; Tarkowski et al., Reference Tarkowski, Witkowska and Opas1977). In addition, two diploid blastomeres can be fused using polyethylene glycol (Eglitis, Reference Eglitis1980; Spindle, Reference Spindle1981), inactivated Sendai virus (O'Neill et al., Reference O'Neill, Speirs and Kaufman1990) or electrofusion (Berg, Reference Berg1982; Kubiak & Tarkowski, Reference Kubiak and Tarkowski1985). Stimulation of 2-cell embryo fusion by electrical pulses appears to be the most efficient method and has been used to produce tetraploid embryos in a number of species including mouse (Kubiak & Tarkowski, Reference Kubiak and Tarkowski1985), rabbit (Ozil & Modlinski, Reference Ozil and Modlinski1986), cow (Iwasaki et al., Reference Iwasaki, Kono, Fukatsu and Nakahara1989; Curnow et al., Reference Curnow, Gunn and Trounson2000), pig (Prather et al., Reference Prather, Hoffman, Schoenbeck, Stumpf and Li1996; Prochazka et al., Reference Prochazka, Vodicka, Zudova, Rybar and Motlik2004) and rat (Krivokharchenko et al., Reference Krivokharchenko, Galat, Ganten and Bader2002).

Although preimplantation development of electrofusion-generated tetraploid embryos has been examined in a number of species, the results of post-implantation development have been limited. In the mouse, the most advanced viable homogenously tetraploid embryo has been recovered on the 15th day of gestation and its morphological features suggest that it was developmentally equivalent to a normal embryo of around 13.5 to 14 days post coitus. (Kaufman & Webb, Reference Kaufman and Webb1990). In contrast, fused tetraploid rabbit embryos generated by an electronic pulse can develop normally at least two-thirds of the way through pregnancy, whereas rabbit embryos electrofused at the 2-cell stage display occasional mosaic preimplantation development (Ozil & Modlinski, Reference Ozil and Modlinski1986).

It has been reported that most mouse tetraploid cells do not contribute to the inner cell mass (ICM) in chimeric embryos with diploid cells at the blastocyst stage, although tetraploid cells tended to colonize in the trophectoderm (Everett & West, Reference Everett and West1996, Reference Everett and West1998; Everett et al., Reference Everett, Stark, West, Davidson and Baldock2000). Furthermore, during postimplantation, although diploid cells contribute to both embryonic and extraembryonic lineages, most tetraploid cells contributed to the extraembryonic lineage (Tarkowski et al., Reference Tarkowski, Witkowska and Opas1977; Nagy et al., Reference Nagy, Gocza, Diaz, Prideaux, Ivanyi, Markkula and Rossant1990; James et al., Reference James, Klerkx, Keighren, Flockhart and West1995; Wang et al., Reference Wang, Kiefer, Urbanek and Wagner1997; Tang & West, Reference Tang and West2000; Goto et al., Reference Goto, Matsui and Takagi2002). Indeed, the aggregation of tetraploid embryos with cells involved in embryonic stem (ES) cells that could not develop independently and injection of these into tetraploid blastocysts allowed the production of mice (Nagy et al., Reference Nagy, Rossant, Nagy, Abramow-Newerly and Roder1993; Ueda et al., Reference Ueda, Jishage, Kamada, Uchida and Suzuki1995; Wang et al., Reference Wang, Kiefer, Urbanek and Wagner1997). Furthermore, in mouse, aggregation of 1/4 and/or 2/8 blastomeres with 2-, 3- or 4-cell carrier tetraploid embryos allowed development to normal and fertile adults, although mouse single ‘quarter’ blastomeres were no longer totipotent, because they were not able to develop independently into mice (Tarkowski et al., Reference Tarkowski, Ozdzenski and Czolowska2001).

In rat, recently, electrofused blastomeres of rat 2-cell embryos were reported to develop to the blastocyst stage in vitro as homogenously as tetraploid embryos (Krivokharchenko et al., Reference Krivokharchenko, Galat, Ganten and Bader2002). However, postimplantation development of rat tetraploid embryos has not been determined. Moreover, it has not been assessed whether rat tetraploid embryos have the ability to support the development of diploid cells that cannot develop independently.

In the present study, we examined the pre-implantation and postimplantation development of rat tetraploid embryos produced by electrofusion of 2-cell-stage embryos. We also examined whether rat tetraploid embryos have the ability to support the development of blastomeres that cannot develop independently.

Materials and methods

Animals

Wistar Imamichi rats were purchased from Japan SLC and bred in our laboratory. GFP-transgenic rats with a CAG (cytomegalovirus enhancer, chicken actin enhancer–promoter and rabbit globin polyA signal) promoter were developed from Wistar rats (Hakamata et al., Reference Hakamata, Tahara, Uchida, Sakuma, Nakamura, Kume, Murakami, Takahashi, Takahashi, Hirabayashi, Ueda, Miyoshi, Kasai and Kobayashi2001; Takeuchi et al., Reference Takeuchi, Sereemaspun, Inagaki, Hakamata, Kaneko, Murakami, Takahashi, Kobayashi and Ookawara2003). Lights were switched on between 9:00 and 21:00 daily. The estrus cycle of females was monitored by daily examination of vaginal smear. Rats with at least three consecutive regular cycles were used in this study. At proestrus, females were caged with males for mating and presence of vaginal plugs and/or sperm in the vaginal smear the next morning was taken to indicate the first day of pregnancy. All procedures adhered to the Guide for the Care and Use of Laboratory Animals published by Tohoku University.

Embryo collection and culture

Embryos were collected as previously described (Matsumoto et al., Reference Matsumoto, Jiang, Mitani and Sato2002a). Early rat 2-cell embryos were collected from mated females at 12:00 on day 2 of pregnancy and were then cultured in 100 µl droplets of mR1ECM medium (Miyoshi et al., Reference Miyoshi, Kono and Niwa1997) overlaid with liquid paraffin (Nacalai Tesque) in a humidified atmosphere of 5% CO2 in air at 37 °C.

Production of tetraploid embryos

For production, 2-cell-stage embryos were placed between the electrodes of a fusion chamber filled with 0.3 M mannitol containing 0.1 mM MgSO4, 0.05 mM CaCl2 and 0.1 mg/ml polyvinyl alcohol at 37 °C. The fusion of 2-cell embryos was induced by an alternating current field (12 V, 500 kHz, 15 s) and two direct current pulses of 1.20 V/cm for 70 µs with a 1 s interval between pulses. The embryos were then placed in a culture droplet and checked every 10 min. Embryos usually fused within 20 min.

Examination of the karyotype of the diploid or tetraploid blastocysts

The karyotype of the diploid or tetraploid blastocysts was examined as described previously with slight modifications (Tarkowski, Reference Tarkowski1966). Briefly, blastocysts were incubated in 0.4 µg/ml demecolcine (Sigma) for 6 h to synchronize the blastocyst cells at metaphase. Next, the blastocysts were cultured in hypotonic solution consisting of 25% culture medium and 75% deionized water for 1 h. Cells were then spread and fixed with glacial acetic acid. Chromosome slides were prepared by air drying and stained with Giemsa. We only examined embryos showing more than five metaphase spread cells to define as either diploid or tetraploid embryo.

Production of two blastomeres in a zona pellucida derived from 8-cell-stage embryos

All micromanipulation procedures were carried out in mR1ECM medium buffered with 10 mM HEPES and 15 mM NaHCO3 and supplemented with 2.4 µg/ml cytochalasin B at room temperature. A pair of blast-omeres at the 8-cell stage were removed from the zona pellucida with a micropipette and separated from each other by gentle pipetting. Each pair of separated blastomeres was then inserted into an evacuated zona pellucida at the 8-cell stage. Manipulated embryos, two blastomeres in a zona pellucida, were cultured as described above.

Production of 2n ↔ 4n chimeric embryos

The production of 2n ↔ 4n chimeric embryos was performed as described previously with slight modifications (Tsunoda et al., Reference Tsunoda, Yasui, Okubo, Nakamura and Sugie1987). One blastomere was removed from a 4-cell-stage 4n(GFP+) embryo using a pipette (20 to 25 µm external diameter) driven by a piezo-actuated unit (Prime Tech). Next, two blastomeres isolated from the 8-cell-stage 2n(GFP−) embryos were inserted into the 4n embryos. As a control, two blastomeres were removed from the 8-cell-stage 2n(GFP+) embryos, followed by insertion of two blastomeres isolated from the 8-cell-stage 2n(GFP−) embryos into the 2n(GFP+) embryos.

Embryo transfer to recipient rats and examination of implantation sites

Embryos at the morula to blastocyst stage were transferred to the uteri of pseudopregnant recipients on day 5. On days 7 to 9, the implantation sites were collected after intravenous injections of Chicago Blue B dye in saline solution (Matsumoto et al., Reference Matsumoto, Ma, Daikoku, Zhao, Paria, Das, Trzaskos and Dey2002b). Small pieces of tissue were fixed with 3.7% formaldehyde and then embedded in paraffin wax. Sections (10 µm) were stained with hematoxylin–eosin. To examine the localization of GFP, immunohistochemical analysis was performed as described previously with slight modifi-cations (Takeuchi et al., Reference Takeuchi, Sereemaspun, Inagaki, Hakamata, Kaneko, Murakami, Takahashi, Kobayashi and Ookawara2003). Deparaffinized sections were incubated sequentially with rabbit anti-GFP antibody (Molecular Probes), biotinylated anti-rabbit IgG antibody (Vector Laboratories) and horseradish peroxidase-conjugated streptavidin (Vector Laboratories). Reactions were visualized using 3-amino-9-ethyl carbazole (Zymed Laboratories) as a chromogen.

Statistical analysis

χ2 analysis was used to evaluate differences. A p-value less than 0.05 was considered significant. Comparisons with expected values of less than 5 were analysed using Fischer's exact probability test.

Results

Development of tetraploid embryos

Developmental rate to the morula/blastocyst stage of tetraploid embryos was 93% (56/60) at 72 h after the start of culture (Table 1). This was not significantly different from that of diploid embryos (95%, 55/58). Compaction in both diploid and tetraploid embryos occurred at 54 h (Fig. 1A, B, D, E). Specifically, diploid embryos compacted at the 8-cell stage (Fig. 1B), whereas compaction of tetraploid embryos occurred at the 4-cell stage (Fig. 1D). Chromosomes examined in all blastocysts that were developed from fused and untreated embryos showed diploid (100%, 30/30) and tetraploid (100%, 21/21) karyotypes, respectively (Fig. 1C, F). After embryo transfer, both diploid and tetraploid embryos showed normal implantation (Fig. 2A, B, F, G) until day 8 of pregnancy, although tetraploid conceptuses were aberrant on days 9 (Fig. 2H) and 10 (Fig. 2I, J).

Figure 1 Preimplantation development of diploid and tetraploid rat embryo in vitro. Untreated (A, B) and fused (D, E) embryos at 48 h (A, D) and 54 h (B, E) after the start of culture. Untreated and fused embryos showed diploid (C) and tetraploid (F) karyotypes, respectively. Note the compaction at 4-cell stage in tetraploid embryos. Bars in (E) and (F) indicate 30 µm and 2 µm, respectively.

Figure 2 Postimplantation development of diploid and tetraploid rat embryos after embryo transfer. Diploid (A–E) and tetraploid (F–J) conceptuses on days 7 (A, F), 8 (B, G), 9 (C, H), 10 (D, I, J) and 11 (e) of pregnancy. Note the aberration in tetraploid embryos on days 9 and 10. Bars in (G) and (J) indicate 150 µm and 1 mm, respectively.

Table 1 Preimplantation development of electrofused tetraploid rat embryos in vitro

Values represent no. (and %).

a Based on the number of 2-cell stage (diploid) or fused embryos (tetraploid).

Development of embryos from two diploid blastomeres isolated at the 8-cell stage

To address whether rat tetraploid embryos have the ability to support the development of diploid cells that cannot develop independently, we examined the developmental potential in pairs of diploid blastomeres isolated at the 8-cell stage. Embryos developed from two diploid blastomeres isolated at the 8-cell stage (Fig. 3A) reached the morula/blastocyst stage (Fig. 3B, C; 89%, 41/46) at 24 h after isolation (at 72 h after the start of culture). Blastocysts appeared as trophectoderm vesicles. The timing of compaction and blastocyst formation in these embryos resembled that of intact 8-cell embryos (72 h after the start of culture). After embryo transfer, implantation sites were identified as blue bands along the uterine horns after injection of a Chicago blue B (Matsumoto et al., Reference Matsumoto, Ma, Daikoku, Zhao, Paria, Das, Trzaskos and Dey2002b). Although the rate of Chicago blue-positive sites was 50% (10/20) on day 7 of pregnancy, only one embryo attached (5%, 1/20; Fig. 3D). On days 8 and 9, the rates of Chicago blue positive sites were 31% (5/16) and 32% (7/22), whereas one degenerated conceptus was obtained on each day (6%, 1/16 and 5%, 1/22; Fig. 3E, F).

Figure 3 Development of embryos from two blastomeres isolated at the 8-cell stage. An isolated pair of blastomeres (A), a morula (B) and a blastocyst (C). Postimplantation development of embryos from two blastomeres isolated at the 8-cell stage after embryo transfer on days 7 (D), 8 (E) and 9 (F) of pregnancy. Bars in (C), (D) and (F) indicate 30 µm, 100 µm and 500 µm, respectively.

Tetraploid embryos support the postimplantation development of two diploid blastomeres isolated at the 8-cell stage

To assess the ability of tetraploid embryos to act as carrier blastomeres, as has been previously demonstrated in the mouse, we examined the development of diploid (GFP−) ↔ tetraploid (GFP+) chimeric embryos. Chimeric rat embryos, in which two diploid blastomeres from an 8-cell embryo were aggregated with three tetraploid blastomeres from a 4-cell embryo, developed to the morula/blastocyst stage (93%, 109/117) at 24 h after the manipulation (72 h after the start of culture; Table 2 and Fig. 4). This did not differ from the development of diploid embryos (100%, 51/51). Analysis of GFP expression showed that the contribution of 4n(GFP+) cells to chimeric blastocysts was mosaic and similar to 2n(GFP−) ↔ 2n(GFP+) embryos (Fig. 4). Our goal was to assess whether the rat tetraploid embryos could support the development of embryos that lacked full developmental potential to term by themselves. We usually estimate the fetal development on days 13–14 after manipulated embryo transfer (Shinozawa et al., Reference Shinozawa, Mizutani, Tomioka, Kawahara, Sasada, Matsumoto and Sato2004). Therefore, we examined the development of chimeric conceptuses and the contribution of tetraploid cells on development on day 14 of pregnancy. On day 14, four conceptuses (4%, 4/109) were obtained (Table 2), although all of them were aberrant and smaller than those of the 2n(GFP−) ↔ 2n(GFP+) chimeric fetuses (Fig. 5A, D).

Table 2 Preimplantation and postimplantation development of chimeric rat embryosa

Implantation and fetus were examined on day 14 of pregnancy. Values represent no. (and %).

a Generated by aggregating a pair of diploid blastomeres from an 8-cell-stage embryo with three tetraploid blastomeres from a 4-cell-stage embryo.

b Carrier of the GFP transgene; IS, implantation sites.

Figure 4 Distribution of GFP-positive cells in chimeric rat embryos. Blastocysts derived from 2n(GFP−) ↔ 2n(GFP+) embryos (A, B) and 2n(GFP−) ↔ 4n(GFP+) embryos (C, D). Bar = 30 µm.

Figure 5 Postimplantation development on day 14 of pregnancy. Fetuses derived from 2n(GFP−) ↔ 2n(GFP+) embryos (A) and 2n(GFP−) ↔ 4n(GFP+) embryos (D). Contribution of GFP(+) cells was assessed by immunohistochemical analysis in 2n(GFP−) ↔ 2n(GFP+) conceptus (B, fetus; C, placenta) and 2n(GFP−) ↔ 4n(GFP+) conceptus (E, fetus; F, placenta). Positive (G) or negative control (H) in 2n(GFP+) conceptus was performed using immunohistochemical analysis with or without primary antibody, respectively. Note that neither fetus nor placenta was GFP-positive in the 2n(GFP−) ↔ 4n(GFP+) conceptus. Bars in (D), (E, H) and (F) indicate 2 mm, 1 mm and 500 µm, respectively. La, labyrinth; Nt, neural tube; T, trophoblastic giant cell.

To examine the localization of 4n(GFP+), immunohistochemical analysis was performed for three conceptuses out of four and showed neither staining for GFP in fetus nor placenta (Fig. 5E, F). These results indicate that rat tetraploid embryos are able to prolong the development of diploid blastomeres that cannot develop independently, although postimplantation development was incomplete.

Discussion

In a previous study in mouse, morphological features of day 15 tetraploid embryos suggested that they were developmentally equivalent to a normal embryo of around 13.5 to 14 days post coitus (Kaufman & Webb, Reference Kaufman and Webb1990). In contrast, rat tetraploid embryos implant normally and survive until day 8 of pregnancy. How-ever, these embryos showed signs of aberrant development on day 9. These results suggest that rat tetraploid embryos are less able to undergo normal development beyond day 8 than those from the mouse. Because compaction of rat tetraploid embryos occurred at the 4-cell stage while diploid embryos compacted at the 8-cell stage, the number of cells in the tetraploid embryos transferred into uteri may be half that in diploid embryos. Therefore, reduced cell number in the tetraploid rat embryos may the cause of aberrant fetal development, although these embryos have the ability to implant.

It has been reported previously that the aggregation of ES cells with tetraploid embryos or injection of ES cells into tetraploid blastocysts has allowed the production of mice that were entirely derived from ES cells (Nagy et al., Reference Nagy, Rossant, Nagy, Abramow-Newerly and Roder1993; Ueda et al., Reference Ueda, Jishage, Kamada, Uchida and Suzuki1995; Wang et al., Reference Wang, Kiefer, Urbanek and Wagner1997). These results suggest that rat tetraploid embryos may also allow the production of rats entirely derived from ES cells. However, rat ES cells that are able to access to germ line have not been established (Iannaccone et al., Reference Iannaccone, Taborn, Garton, Caplice and Brenin1994; Brenin et al., Reference Brenin, Look, Bader, Hubner, Levan and Iannaccone1997; Buehr et al., Reference Buehr, Nichols, Stenhouse, Mountford, Greenhalgh, Kantachuvesiri, Brooker, Mullins and Smith2003). In contrast, in mouse, aggregation of 1/4 and/or 2/8 blastomeres with 2-, 3- or 4-cell carrier tetraploid embryos has allowed development to normal and fertile adult, although mouse single ‘quarter’ blastomeres are no longer totipotent, because they are not able to develop independently into a mouse (Tarkowski et al., Reference Tarkowski, Ozdzenski and Czolowska2001). These results suggest that rat tetraploid embryos may have the ability to support the development of blastomeres that cannot develop independently. However, developmental potential of isolated rat blastomeres from early-stage embryos has not been well understood. In the present study, our results showed that a pair of rat diploid blastomeres isolated at the 8-cell stage developed to the morula/blastocyst stage, while the ability of implantation and postimplantation development was very poor. Developed blastocysts appeared to resemble trophectoderm vesicles without a clear inner cell mass. Therefore, developmental failure of these embryos may be due to lack of sufficient number of ICM cells.

To assess whether the rat tetraploid embryos possess the ability to support the poor developmental potential in a pair of rat diploid blastomeres isolated at the 8-cell stage, we produced chimeric 2n(GFP−) ↔ 4n(GFP+) rat embryos. After transfer 2n(GFP−) ↔ 4n(GFP+) chimeric embryos into uteri, all of the conceptuses obtained on day 14 of pregnancy (four conceptuses) were aberrant and smaller than the 2n(GFP−) ↔ 2n(GFP+) chimeric fetuses. Immuno-histochemical analysis showed neither fetus nor placenta contained GFP-positive cells, although GFP expression showed that the contribution of 4n(GFP+) cells to chimeric blastocysts was mosaic and similar to 2n(GFP−) ↔ 2n(GFP+) embryos. These results suggest that rat tetraploid embryos are able to prolong the development of a pair of diploid blastomeres from the 8-cell blastomeres, although it is incomplete.

In mouse, during preimplantation development, most tetraploid cells do not contribute to the inner cell mass in chimeric embryos with diploid cells at the blastocyst stage, although tetraploid cells tended to colonize in the trophectoderm (Everett & West, Reference Everett and West1996, Reference Everett and West1998; Everett et al., Reference Everett, Stark, West, Davidson and Baldock2000). During postimplantation development, tetraploid cells are abundant in extraembryonic tissues in 2n ↔ 4n aggregation chimeras, whereas they do not contribute to embryonic tissue (Tarkowski et al., Reference Tarkowski, Witkowska and Opas1977; Nagy et al., Reference Nagy, Gocza, Diaz, Prideaux, Ivanyi, Markkula and Rossant1990; James et al., Reference James, Klerkx, Keighren, Flockhart and West1995; Everett & West, Reference Everett and West1996). Although the mechanism by which the developmental potential of tetraploid cells supports the development of diploid cells is not clearly understood, it has been reported that the tendency of tetraploid cells to colonize the trophectoderm occurs at the blastocyst stage and this colonization may be accompanied by selection against tetraploid cells in ICM in mouse (Everett & West, Reference Everett and West1996, Reference Everett and West1998; Everett et al., Reference Everett, Stark, West, Davidson and Baldock2000). In the present study in rat, both ICM and trophectoderm in chimeric blastocysts contained tetraploid cells with mosaic contribution during preimplantation development. Furthermore, our results showed rat tetraploid embryos are less able to undergo postimplantation development compared with mouse. Therefore, poor postimplantation development with different localization of rat tetraploid blastomeres could be associated with quite low developmental rate to chimeric fetus with aberrant and smaller size.

In conclusion, our results suggest that rat tetraploid embryos are able to prolong the development of diploid blastomeres that cannot develop independently, although postimplantation development was incomplete. In chimeric embryos, a different contribution of tetraploid cells compared with that of the mouse may be a cause of incomplete developmental support during postimplantation. Furthermore, the contribution of tetraploid and diploid cells to blastocysts may involve the postimplantation development stage. These results suggest that rat electrofused tetraploid embryos may not allow the development of rats that have been entirely derived from ES cells, if rat ES cells were established. It could be possible that improvement of the fusion procedure to create rat tetraploid embryos and/or culture system for rat embryos increases the ability of tetraploid embryos to act as carrier blastomeres during postimplantation development. Whereas an aberrant and smaller size could account for the lack of tetraploid cells that could develop into either the fetus or placenta on day 14 of pregnancy, it may be possible that they have just ceased to express GFP. Further investigation using other genetic markers might clarify this point.

Acknowledgements

This work was supported by the Japan Society for the Promotion of Science Grant JSPS-16108003 (to E.S.). This work was also supported in part by research grants from the JSPS-17780207, Inamori Foundation and Ito Foundation (to H.M.) and Joint project of Japan–U.S. Cooperative Science Program, JSPS-AGR10002 (to E.S.).

References

Berg, H. (1982). Fusion of blastomeres and blastocysts of mouse embryos. Bioelectrochem. Bioenerg. 9, 223–8.CrossRefGoogle Scholar
Brenin, D., Look, J., Bader, M., Hubner, N., Levan, G. & Iannaccone, P. (1997). Rat embryonic stem cells: a progress report. Transplant. Proc. 29, 1761–5.CrossRefGoogle ScholarPubMed
Buehr, M., Nichols, J., Stenhouse, F., Mountford, P., Greenhalgh, C.J., Kantachuvesiri, S., Brooker, G., Mullins, J. & Smith, A.G. (2003). Rapid loss of Oct-4 and pluripotency in cultured rodent blastocysts and derivative cell lines. Biol. Reprod. 68, 222–9.CrossRefGoogle ScholarPubMed
Curnow, E.C., Gunn, I.M. & Trounson, A.O. (2000). Electrofusion of two-cell bovine embryos for the production of tetraploid blastocysts in vitro. Mol. Reprod. Dev. 56, 372–7.3.0.CO;2-W>CrossRefGoogle ScholarPubMed
Edwards, R.G. (1958). Colchicine-induced heteroploidy in the mouse. II. The induction of tetraploidy and other types of heteroploidy. J. Exp. Zool. 137, 349–62.CrossRefGoogle ScholarPubMed
Eglitis, M.A. (1980). Formation of tetraploid mouse blastocysts following blastomere fusion with polyethylene glycol. J. Exp. Zool. 213, 309–13.CrossRefGoogle ScholarPubMed
Everett, C.A. & West, J.D. (1996). The influence of ploidy on the distribution of cells in chimaeric mouse blastocysts. Zygote 4, 5966.CrossRefGoogle ScholarPubMed
Everett, C.A. & West, J.D. (1998). Evidence for selection against tetraploid cells in tetraploid ↔ diploid mouse chimaeras before the late blastocyst stage. Genet. Res. 72, 225–8.CrossRefGoogle ScholarPubMed
Everett, C.A., Stark, M.H., West, J.D., Davidson, D. & Baldock, R.A. (2000). Three-dimensional reconstruction of tetra-ploid ↔ diploid chimaeric mouse blastocysts. J. Anat. 196, 341–6.CrossRefGoogle Scholar
Goto, Y., Matsui, J. & Takagi, N. (2002). Developmental potential of mouse tetraploid cells in diploid ↔ tetraploid chimeric embryos. Int. J. Dev. Biol. 46, 741–5.Google ScholarPubMed
Hakamata, Y., Tahara, K., Uchida, H., Sakuma, Y., Nakamura, M., Kume, A., Murakami, T., Takahashi, M., Takahashi, R., Hirabayashi, M., Ueda, M., Miyoshi, I., Kasai, N. & Kobayashi, E. (2001). Green fluorescent protein-transgenic rat: a tool for organ transplantation research. Biochem. Biophys. Res. Commun. 286, 779–85.CrossRefGoogle Scholar
Iannaccone, P.M., Taborn, G.U., Garton, R.L., Caplice, M.D. & Brenin, D.R. (1994). Pluripotent embryonic stem cells from the rat are capable of producing chimeras. Dev. Biol. 163, 288–92.CrossRefGoogle ScholarPubMed
Iwasaki, S., Kono, T., Fukatsu, H. & Nakahara, T. (1989). Production of bovine tetraploid embryos by electrofusion and their developmental capability in vitro. Gamete Res. 24, 261–7.CrossRefGoogle ScholarPubMed
James, R.M., Klerkx, A.H., Keighren, M., Flockhart, J.H. & West, J.D. (1995). Restricted distribution of tetraploid cells in mouse tetraploid ↔ diploid chimaeras. Dev. Biol. 167, 213–26.CrossRefGoogle ScholarPubMed
Kaufman, M.H. & Webb, S. (1990). Postimplantation development of tetraploid mouse embryos produced by electrofusion. Development 110, 1121–32.CrossRefGoogle ScholarPubMed
Krivokharchenko, A., Galat, V., Ganten, D. & Bader, M. (2002). In vitro formation of tetraploid rat blastocysts after fusion of two-cell embryos. Mol. Reprod. Dev. 61, 460–5.CrossRefGoogle ScholarPubMed
Kubiak, J.Z. & Tarkowski, A.K. (1985). Electrofusion of mouse blastomeres. Exp. Cell Res. 157, 561–6.CrossRefGoogle ScholarPubMed
Matsumoto, H., Jiang, J.Y., Mitani, D. & Sato, E. (2002 a). Distribution and gene expression of cytoskeletal proteins in two-cell rat embryos and developmental arrest. J. Exp. Zool. 293, 641–8.CrossRefGoogle ScholarPubMed
Matsumoto, H., Ma, W.G., Daikoku, T., Zhao, X., Paria, B.C., Das, S.K., Trzaskos, J.M. & Dey, S.K. (2002 b). Cyclooxygenase-2 differentially directs uterine angiogenesis during implantation in mice. J. Biol. Chem. 277, 29260–7.CrossRefGoogle ScholarPubMed
Miyoshi, K., Kono, T. & Niwa, K. (1997). Stage-dependent development of rat 1-cell embryos in a chemically defined medium after fertilization in vivo and in vitro. Biol. Reprod. 56, 180–5.CrossRefGoogle Scholar
Nagy, A., Gocza, E., Diaz, E.M., Prideaux, V.R., Ivanyi, E., Markkula, M. & Rossant, J. (1990). Embryonic stem cells alone are able to support fetal development in the mouse. Development 110, 815–21.CrossRefGoogle ScholarPubMed
Nagy, A., Rossant, J., Nagy, R., Abramow-Newerly, W. & Roder, J.C. (1993). Derivation of completely cell culture-derived mice from early-passage embryonic stem cells. Proc. Natl. Acad. Sci. U.S.A. 90, 8424–8.CrossRefGoogle ScholarPubMed
O'Neill, G.T., Speirs, S. & Kaufman, M.H. (1990). Sex-chromosome constitution of postimplantation tetraploid mouse embryos. Cytogenet. Cell Genet. 53, 191–5.CrossRefGoogle ScholarPubMed
Ozil, J.P. & Modlinski, J.A. (1986). Effects of electric field on fusion rate and survival of 2-cell rabbit embryos. J. Embryol. Exp. Morphol. 96, 211–28.Google ScholarPubMed
Prather, R.S., Hoffman, K.E., Schoenbeck, R.A., Stumpf, T.T. & Li, J. (1996). Characterization of DNA synthesis during the 2-cell stage and the production of tetraploid chimeric pig embryos. Mol. Reprod. Dev. 45, 3842.3.0.CO;2-T>CrossRefGoogle ScholarPubMed
Prochazka, R., Vodicka, P., Zudova, D., Rybar, R. & Motlik, J. (2004). Development of in vivo derived diploid and tetraploid pig embryos in a modified medium NCSU 37. Theriogeneology 62, 155–64.CrossRefGoogle Scholar
Shinozawa, T., Mizutani, E., Tomioka, I., Kawahara, M., Sasada, H., Matsumoto, H. & Sato, E. (2004). Differential effect of recipient cytoplasm for microtubule organization and preimplantation development in rat reconstituted embryos with two-cell embryonic cell nuclear transfer. Mol. Reprod. Dev. 68, 313–8.CrossRefGoogle ScholarPubMed
Snow, M.H. (1973). Tetraploid mouse embryos produced by cytochalasin B during cleavage. Nature 244, 513–5.CrossRefGoogle ScholarPubMed
Spindle, A. (1981). Polyethylene glycol-induced fusion of two-cell mouse embryo blastomeres. Exp. Cell Res. 131, 465–70.CrossRefGoogle ScholarPubMed
Takeuchi, K., Sereemaspun, A., Inagaki, T., Hakamata, Y., Kaneko, T., Murakami, T., Takahashi, M., Kobayashi, E. & Ookawara, S. (2003). Morphologic characterization of green fluorescent protein in embryonic, neonatal and adult transgenic rats. Anat. Rec. 274A, 883–6.CrossRefGoogle Scholar
Tang, P.C. & West, J.D. (2000). The effects of embryo stage and cell number on the composition of mouse aggregation chimaeras. Zygote 8, 235–43.CrossRefGoogle ScholarPubMed
Tarkowski, A.K. (1966). An air-drying method for chromosome preparations from mouse eggs. Cytogenetics 5, 394400.CrossRefGoogle Scholar
Tarkowski, A.K., Witkowska, A. & Opas, J. (1977). Development of cytochalasin B-induced tetraploid and diploid/tetraploid mosaic mouse embryos. J. Embryol. Exp. Morphol. 41, 4764.Google ScholarPubMed
Tarkowski, A.K., Ozdzenski, W. & Czolowska, R. (2001). Mouse singletons and twins developed from isolated diploid blastomeres supported with tetraploid blastomeres. Int. J. Dev. Biol. 45, 591–6.Google ScholarPubMed
Tsunoda, Y., Yasui, T., Okubo, Y., Nakamura, K. & Sugie, T. (1987). Development one or two blastomeres from eight-cell mouse embryos to term in the presence of parthenogenetic eggs. Theriogenology 28, 615–23.CrossRefGoogle ScholarPubMed
Ueda, O., Jishage, K., Kamada, N., Uchida, S. & Suzuki, H. (1995). Production of mice entirely derived from embryonic stem (ES) cell with many passages by coculture of ES cells with cytochalasin B induced tetraploid embryos. Exp. Anim. 44, 205–10.CrossRefGoogle Scholar
Wang, Z.Q., Kiefer, F., Urbanek, P. & Wagner, E.F. (1997). Generation of completely embryonic stem cell-derived mutant mice using tetraploid blastocyst injection. Mech. Dev. 62, 137–45.CrossRefGoogle ScholarPubMed
Figure 0

Figure 1 Preimplantation development of diploid and tetraploid rat embryo in vitro. Untreated (A, B) and fused (D, E) embryos at 48 h (A, D) and 54 h (B, E) after the start of culture. Untreated and fused embryos showed diploid (C) and tetraploid (F) karyotypes, respectively. Note the compaction at 4-cell stage in tetraploid embryos. Bars in (E) and (F) indicate 30 µm and 2 µm, respectively.

Figure 1

Figure 2 Postimplantation development of diploid and tetraploid rat embryos after embryo transfer. Diploid (A–E) and tetraploid (F–J) conceptuses on days 7 (A, F), 8 (B, G), 9 (C, H), 10 (D, I, J) and 11 (e) of pregnancy. Note the aberration in tetraploid embryos on days 9 and 10. Bars in (G) and (J) indicate 150 µm and 1 mm, respectively.

Figure 2

Table 1 Preimplantation development of electrofused tetraploid rat embryos in vitro

Figure 3

Figure 3 Development of embryos from two blastomeres isolated at the 8-cell stage. An isolated pair of blastomeres (A), a morula (B) and a blastocyst (C). Postimplantation development of embryos from two blastomeres isolated at the 8-cell stage after embryo transfer on days 7 (D), 8 (E) and 9 (F) of pregnancy. Bars in (C), (D) and (F) indicate 30 µm, 100 µm and 500 µm, respectively.

Figure 4

Table 2 Preimplantation and postimplantation development of chimeric rat embryosa

Figure 5

Figure 4 Distribution of GFP-positive cells in chimeric rat embryos. Blastocysts derived from 2n(GFP−) ↔ 2n(GFP+) embryos (A, B) and 2n(GFP−) ↔ 4n(GFP+) embryos (C, D). Bar = 30 µm.

Figure 6

Figure 5 Postimplantation development on day 14 of pregnancy. Fetuses derived from 2n(GFP−) ↔ 2n(GFP+) embryos (A) and 2n(GFP−) ↔ 4n(GFP+) embryos (D). Contribution of GFP(+) cells was assessed by immunohistochemical analysis in 2n(GFP−) ↔ 2n(GFP+) conceptus (B, fetus; C, placenta) and 2n(GFP−) ↔ 4n(GFP+) conceptus (E, fetus; F, placenta). Positive (G) or negative control (H) in 2n(GFP+) conceptus was performed using immunohistochemical analysis with or without primary antibody, respectively. Note that neither fetus nor placenta was GFP-positive in the 2n(GFP−) ↔ 4n(GFP+) conceptus. Bars in (D), (E, H) and (F) indicate 2 mm, 1 mm and 500 µm, respectively. La, labyrinth; Nt, neural tube; T, trophoblastic giant cell.