Size regulation in the mouse embryo

The study describes an analysis of the development of mouse embryos halved at the 2-cell stage by the destruction of one blastomere, in comparison with control embryos of parallel derivation, at 2·5–13·5 days post coitum. The results showed that: (1) half embryos achieve size regulation some time between 7·5 and 10·5 days; (2) there is an indication that by 13·5 days half embryos may have again dropped back significantly in size relative to controls; (3) preregulation half embryos are slightly retarded developmental, but this does not wholly account for their smaller size: morphogenesis is not size-dependent; (4) early postimplantation half embryos contain a significantly decreased proportion of inner cell mass derivatives and increased proportion of trophectoderm derivatives when compared with controls. A comparison is also made between the up-regulation of half embryos and the down-regulation of aggregate embryos, and it is suggested that size regulation may occur by delaying a change in the normal growth rate.

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Size regulation in the mouse embryo

Development ◽

10.1242/dev.94.1.139 ◽

1986 ◽

Vol 94 (1) ◽

pp. 139-148

Author(s):

G. F. Rands

Keyword(s):

Mouse Embryo ◽

Inner Cell Mass ◽

Cell Mass ◽

Nutrient Supply ◽

Mouse Embryos ◽

Down Regulation ◽

Cell Stage ◽

Size Regulation ◽

Internal Cavities

The development of mouse embryos formed by the aggregation of four 8-cell-stage eggs was analysed in comparison with control single embryos. The analysis revealed that: (1) Quadruple aggregates undergo size regulation over several days, starting before implantation and being completed by 6·5 days post coitum. (2) The attainment of recognizable postimplantation morphological stages is independent of size. (3) Regulation is not brought about by disproportionate alterations in the size of the internal cavities. (4) Regulation in both inner cell mass (ICM) and trophectoderm derivatives is completed between 5·5 and 6·5 days post coitum. (5) Despite the abnormal proportions of ICM and trophectoderm in quadruple blastocysts, the proportions of the tissues derived from them are already normal by 5·5 days. The possibility that down regulation in size of aggregate embryos occurs as a consequence of limited nutrient supply is discussed.

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The nature and distribution of serologically detectable alloantigens on the preimplantation mouse embryo

Development ◽

10.1242/dev.35.1.59 ◽

1976 ◽

Vol 35 (1) ◽

pp. 59-72

Author(s):

Audrey L. Muggleton-Harris ◽

Martin H. Johnson

Keyword(s):

Mouse Embryo ◽

Inner Cell Mass ◽

Cell Mass ◽

Convincing Evidence ◽

Mouse Embryos ◽

Cell Type ◽

Cell Stage ◽

Preimplantation Mouse Embryos ◽

Preimplantation Mouse Embryo ◽

Preimplantation Mouse

The nature and distribution of surface alloantigens on preimplantation mouse embryos has been examined by immunofluorescence. Non-H-2 alloantigens were detected at allstages examined, from the 2-cell to the 4½-day blastocyst. Cleaving blastomeres, inner cell mass cells and cells of the primary trophectoderm were all positive. In F1 embryos maternalnon-H-2 alloantigens were detectable at all stages, whereas paternal antigens first became evident at the 6- to 8-cell stage. No convincing evidence of the presence of alloantigens associated with the H-2 haplotype was found at any stage or on any cell type, suggesting that if these antigens are present they are in low quantity or are masked.

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Totipotency of mouse zygotes extends to single blastomeres of embryos at the four-cell stage

Scientific Reports ◽

10.1038/s41598-021-90653-1 ◽

2021 ◽

Vol 11 (1) ◽

Author(s):

Marino Maemura ◽

Hiroaki Taketsuru ◽

Yuki Nakajima ◽

Ruiqi Shao ◽

Ayaka Kakihara ◽

...

Keyword(s):

Inner Cell Mass ◽

Cell Mass ◽

Mouse Embryos ◽

Primitive Endoderm ◽

Cell Stage ◽

Supportive Environment ◽

Mouse Zygotes ◽

Single Blastomeres ◽

Multicellular Organisms

AbstractIn multicellular organisms, oocytes and sperm undergo fusion during fertilization and the resulting zygote gives rise to a new individual. The ability of zygotes to produce a fully formed individual from a single cell when placed in a supportive environment is known as totipotency. Given that totipotent cells are the source of all multicellular organisms, a better understanding of totipotency may have a wide-ranging impact on biology. The precise delineation of totipotent cells in mammals has remained elusive, however, although zygotes and single blastomeres of embryos at the two-cell stage have been thought to be the only totipotent cells in mice. We now show that a single blastomere of two- or four-cell mouse embryos can give rise to a fertile adult when placed in a uterus, even though blastomere isolation disturbs the transcriptome of derived embryos. Single blastomeres isolated from embryos at the eight-cell or morula stages and cultured in vitro manifested pronounced defects in the formation of epiblast and primitive endoderm by the inner cell mass and in the development of blastocysts, respectively. Our results thus indicate that totipotency of mouse zygotes extends to single blastomeres of embryos at the four-cell stage.

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Abnormal development of pre-implantation mouse embryos grown in vitro with [3H]thymidine

Development ◽

10.1242/dev.29.3.601 ◽

1973 ◽

Vol 29 (3) ◽

pp. 601-615

Author(s):

M. H. L. Snow

Keyword(s):

Specific Activity ◽

Inner Cell Mass ◽

Cell Damage ◽

Cell Mass ◽

Cell Number ◽

Mouse Embryos ◽

Abnormal Development ◽

Tritium Concentration ◽

Cell Stage

Mouse embryos were grown in vitro from the 2-cell stage to blastocysts in the presence of [3H]thymidine. Methyl-T-thymidine and thymidine-6-T(n) were used and both forms found to be lethal at concentrations above 0·1 μCi/ml. Both forms of [3H]Tdr at concentrations between 0·01 and 0·1 μCi/ml caused a highly significant (P < 0·001) reduction in blastocyst cell number. The reduction in cell number, which was positively correlated with specific activity and tritium concentration, was associated with cell damage typical of radiation damage caused by tritium disintegration. Thymidine-6-T(n) also significantly reduced the number of 2-cell embryos forming blastocysts whereas methyl-T-Tdr did not. This difference in effect is assumed to be caused by contamination of one form of [3H]Tdr with a by-product of the tritiation process. A study of the cleavage stages showed that almost all the reduction in cell numbers could be accounted for by selective cell death occurring at the 16-cell stage. Cells which survive that stage cleave at a normal rate. The cells that are most susceptible to [3H]Tdr damage were found to normally contribute to the inner cell mass. The [3H]Tdr-resistant cells form the trophoblast. It is possible to grow blastocysts in [3H]Tdr such that they contain no inner cell mass but are composed entirely of trophoblast. Comparatively short (12 h) incubation with [3H]Tdr at any stage prior to the 16-cell stage will cause this damage. Possible reasons for this differential effect are discussed, and also compared with damage caused by X-irradiation.

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Potential of two-cell mouse embryos to develop to term despite partial damage after cryopreservation

Laboratory Animals ◽

10.1258/002367795781088252 ◽

1995 ◽

Vol 29 (3) ◽

pp. 320-326 ◽

Cited By ~ 14

Author(s):

Th. Rülicke ◽

P. Autenried

Keyword(s):

Inner Cell Mass ◽

Cell Mass ◽

Blastocyst Stage ◽

Mouse Embryos ◽

Cell Stage ◽

Freeze Thaw ◽

Foster Mothers ◽

Vital Stains ◽

Partial Damage

Approximately 18% of cryopreserved 2-cell mouse embryos of 26 different batches showed various degrees of morphological damage after the freeze-thaw process. Normal and damaged morphology were assessed by light microscopy and the ability of an embryo to develop in vitro to a blastocyst, or to develop to term, after transfer to foster mothers. Using vital stains such as Fluorescein-diacetate (FDA) and 4',6-Diamidino-2-Phenylindole (DAPI) it was found that in approximately 82% of the cases, both of the 2 blastomeres of the cryopreserved embryos survived the freeze-thaw process; in 10% only one cell survived the process; and in 8% none survived. Normally, only intact 2-cell embryos are considered for transfer. Here it was shown that over 60% of the partially damaged embryos developed in vitro to the blastocyst stage and, of those, 26% developed to term after transfer to suitable foster mothers. Although the inner cell mass (ICM) appeared to remain smaller during culture after the transfer of partially damaged 2-cell stage embryos, no difference during gestation period was found compared with intact embryos.

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Developmental pattern of hexaploid mouse embryos produced by blastomere fusion of diploid and tetraploid embryos at the 2-cell stage

Zygote ◽

10.1017/s0967199409005206 ◽

2009 ◽

Vol 17 (2) ◽

pp. 125-130 ◽

Cited By ~ 2

Author(s):

Lei Lei ◽

Na Guan ◽

Yan-Ning Xu ◽

Qing-Hua Zhang ◽

Jing-Ling Shen ◽

...

Keyword(s):

Inner Cell Mass ◽

Karyotype Analysis ◽

Cell Mass ◽

Cell Number ◽

Blastocyst Stage ◽

Lower Number ◽

Mouse Embryos ◽

Developmental Pattern ◽

Cell Stage ◽

Positive Expression

SummaryPolyploid mouse embryos are important models for understanding the mechanisms of cleavage and preimplantation development in mammals. In this study, hexaploid (6n) mouse embryos were produced by the electrofusion of blastomeres from diploid (2n) and tetraploid (4n) embryos at the 2-cell stage. Furthermore, the developmental pattern of hexaploid embryos was evaluated by blastocyst rate, cell number, karyotype analysis, cytoskeleton staining and Oct-4 immunofluorescence. The results showed that 72.7% of the hexaploid embryos were able to develop to the blastocyst stage, which is a lower number than that found with normal diploid embryos (98.0%, p < 0.05). The cell number in hexaploid blastocyst was 12.3 ± 2.0, which was less than that found in diploid or tetraploid blastocysts (41.2 ± 7.2; 18.4 ± 3.5). Karyotype analysis confirmed that the number of chromosomes in hexaploid embryos was 120. β-Tubulin and Oct-4 immunofluorescence indicated that the hexaploid blastocysts were nearly lacking inner cell mass (ICM), but some blastomeres did show Oct-4-positive expression.

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Tissue-specific control of expression of the tight junction polypeptide ZO-1 in the mouse early embryo

Development ◽

10.1242/dev.113.1.295 ◽

1991 ◽

Vol 113 (1) ◽

pp. 295-304 ◽

Cited By ~ 5

Author(s):

T.P. Fleming ◽

M.J. Hay

Keyword(s):

Tight Junction ◽

Contact Area ◽

Inner Cell Mass ◽

Cell Mass ◽

Subsequent Development ◽

Early Embryo ◽

Cell Contact ◽

Down Regulation ◽

Cell Stage ◽

Daughter Cells

The processes governing differential protein expression in preimplantation lineages were investigated using a monoclonal antibody recognising the tight junction polypeptide, ZO-1. ZO-1 localises to the maturing tight junction membrane domain in the polarised trophectoderm lineage from compaction (8-cell stage) onwards, ultimately forming a zonular belt around each trophectoderm cell of the blastocyst (32- to 64-cell stage). The protein is usually undetectable within the inner cell mass (ICM) although, in a minority of embryos, punctate ZO-1 sites are present on the surface of one or more ICM cells. Since ICM cells derive from the differentiative division of polarised 8- and 16-cell blastomeres, the distribution of ZO-1 following differentiative division in isolated, synchronised cell clusters of varying size, was examined. In contrast to the apical cytocortical pole, ZO-1 was found to be inherited by nonpolar (prospective ICM) as well as polar (prospective trophectoderm) daughter cells. Following division, polar cells adhere to and gradually envelop nonpolar cells. Prior to envelopment, ZO-1 localises to the boundary between the contact area and free membrane of daughter cells, irrespective of their phenotype. After envelopment, polar cells retain these ZO-1 contact sites whilst nonpolar cells lose them, in which case ZO-1 transiently appears as randomly-distributed punctate sites on the membrane before disappearing. Thus, symmetrical cell contact appears to initiate ZO-1 down-regulation in the ICM lineage. The biosynthetic level at which ZO-1 down-regulation occurs was investigated in immunosurgically isolated ICMs undergoing trophectoderm regeneration. By 6 h in culture, isolated ICMs generated a zonular network of ZO-1 at the contact area between outer cells, thereby demonstrating the reversibility of down-regulation. This assembly process was unaffected by alpha-amanitin treatment but was inhibited by cycloheximide. These results indicate that the ICM inherits and stabilises ZO-1 transcripts which can be utilised for rapid synthesis and assembly of the protein, a capacity that may have significance both in maintaining lineage integrity within the blastocyst and in the subsequent development of the ICM.

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Gp330 is specifically expressed in outer cells during epithelial differentiation in the preimplantation mouse embryo

Development ◽

10.1242/dev.120.11.3289 ◽

1994 ◽

Vol 120 (11) ◽

pp. 3289-3299 ◽

Cited By ~ 3

Author(s):

C. Gueth-Hallonet ◽

A. Santa-Maria ◽

P. Verroust ◽

B. Maro

Keyword(s):

Mouse Embryo ◽

Inner Cell Mass ◽

Cell Mass ◽

Blastocyst Stage ◽

Transcriptional Level ◽

Cell Stage ◽

Preimplantation Mouse ◽

Extensive Cell ◽

High Level ◽

Endocytic Activity

During preimplantation development of the mouse embryo, a layer of outer cells differentiates into a perfect epithelium, the trophectoderm. The divergence between the trophectoderm and the inner cell mass takes place from the 8-cell stage to the 64-cell stage and precedes their commitment at the blastocyst stage. In this work, we have investigated the expression of gp330, a 330 × 10(3) M(r) glycoprotein found in clathrin-coated areas of the plasma membrane of some epithelial cells characterized by a high level of endocytic activity. Our results show that gp330 is first synthesized in 16-cell stage embryos and that its appearance is restricted to outer cells until the blastocyst stage. Furthermore, its expression is repressed in inner cells at a post-transcriptional level, probably through the development of extensive cell-cell contacts.

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Cytokeratin filament assembly in the preimplantation mouse embryo

Development ◽

10.1242/dev.101.3.565 ◽

1987 ◽

Vol 101 (3) ◽

pp. 565-582 ◽

Cited By ~ 7

Author(s):

J.C. Chisholm ◽

E. Houliston

Keyword(s):

Mouse Embryo ◽

Inner Cell Mass ◽

Cell Mass ◽

Blastocyst Stage ◽

Lineage Tracing ◽

Cell Stage ◽

Filament Assembly ◽

Filament Networks ◽

Tracing Techniques ◽

Cytokeratin Filaments

The timing, spatial distribution and control of cytokeratin assembly during mouse early development has been studied using a monoclonal antibody, TROMA-1, which recognizes a 55,000 Mr trophectodermal cytokeratin (ENDO A). This protein was first detected in immunoblots at the 4-cell stage, and became more abundant at the 16-cell stage and later. Immunofluorescence analysis revealed assembled cytokeratin filaments in some 8-cell blastomeres, but not at earlier stages. At the 16-cell stage, filaments were found in both polarized (presumptive trophectoderm; TE) and apolar (presumptive inner cell mass; ICM) cells in similar proportions, although polarized cells possessed more filaments than apolar cells. By the late 32-cell, early blastocyst, stage, all polarized (TE) cells contained extensive filament networks whereas cells positioned inside the embryo tended to have lost their filaments. The presence of filaments in inside cells at the 16-cell stage and in ICM cells was confirmed by immunoelectron microscopy. Lineage tracing techniques demonstrated that those cells in the ICM of early blastocysts which did possess filaments were almost exclusively the progeny of polar 16-cell blastomeres, suggesting that these filaments were directly inherited from outside cells at the 16- to 32-cell transition. Inhibitor studies revealed that proximate protein synthesis but not mRNA synthesis is required for filament assembly at the 8-cell stage. These results demonstrate that there are quantitative rather than qualitative differences in the expression of cytokeratin filaments in the inner cell mass and trophectoderm cells of the mouse embryo.

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Membrane organization in the preimplantation mouse embryo

Development ◽

10.1242/dev.90.1.101 ◽

1985 ◽

Vol 90 (1) ◽

pp. 101-121

Author(s):

Hester P. M. Pratt

Keyword(s):

Mouse Embryo ◽

Inner Cell Mass ◽

Cell Mass ◽

Freeze Fracture ◽

Molecular Organization ◽

Surface Polarity ◽

Cell Stage ◽

Preimplantation Mouse Embryo ◽

Preimplantation Mouse ◽

Polarized Epithelium

The preimplantation mouse blastocyst consists of two differentiated tissues, the trophectoderm (a structurally and functionally polarized epithelium) and the inner cell mass. The divergence of these two cell types can be traced back to a contact dependent polarization of the surface and cytoplasm at the 8-cell stage. Membrane/cytocortical organization during this preimplantation period has been studied using freeze fracture in conjunction with the sterol-binding antibiotic filipin in an attempt to discern the molecular basis and origin of these surface asymmetries. The distribution of filipin reactivity within the different membrane domains showed that the surface polarity exhibited by trophectoderm and by blastomeres of the 8-cell stage is underlain by a heterogeneity in molecular organization of the membrane/cytocortex which may originate prior to the appearance of any overt surface polarity. The results are discussed in terms of the likely basis of this membrane/cytocortical asymmetry, its probable origins and the use of the preimplantation mouse embryo as a model system for studying the assembly of a polarized epithelium.

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