Wrenzycki C, Herrmann D, Carnwath J W, Niemann H
Department of Biotechnology, Institut für Tierzucht und Tierverhalten (FAL), Mariensee, Neustadt, Germany.
J Reprod Fertil. 1998 Mar;112(2):387-98. doi: 10.1530/jrf.0.1120387.
This study investigated the effects of a semi-defined culture system on the temporal pattern of expression of RNA from genes involved in compaction and cavitation: gap junction protein connexin43 (Cx43), desmosomal glycoproteins desmoglein 1 (Dg 1), desmocollins I, II and III (Dc I, Dc II, Dc III), desmosomal protein plakophilin (Plako); metabolism glucosetransporter-1 (Glut-1); RNA processing poly(A)polymerase (PolyA); heat shock protein 70.1 (HSP); and trophoblastic function trophoblast protein (TP) in bovine oocytes and embryos generated in vitro using TCM199 supplemented with BSA as the culture medium. Morulae and blastocysts derived in vivo were collected from superovulated heifers and also used for this study. Poly(A)+ RNA was extracted from pools of 20-50 oocytes or embryos, analysed by reverse transcription-polymerase chain reaction and the amplified fragments were verified by sequencing. Assays were repeated at least three times for each developmental stage and provided consistent results in all replicates. In bovine embryos produced in vitro, mRNA encoding Cx43 was detectable up to the morula stage, whereas blastocysts and hatched blastocysts did not express this gene. No transcripts were found for Dg 1 and Dc I throughout the tested preimplantation stages. Dc II and Dc III transcripts were found from 2-4-cell embryos up to the hatched blastocyst stage. mRNA encoding Plako was detected in immature and mature oocytes and zygotes, while no transcripts were seen in 2-4-cell and 8-16-cell embryos. The gene was expressed again from the morulae to the hatched blastocyst stage. Oocytes and bovine embryos produced in vitro showed transcripts for Glut-1, PolyA and HSP throughout preimplantation development up to the hatched blastocyst stage. The gene encoding TP was transcribed only in blastocysts and hatched blastocysts. Morulae and blastocysts produced in vivo showed the same expression as their in vitro counterparts, with one exception: the in vivo embryos transcribed Cx43. The results of this study reveal for the first time the transcriptional pattern of a set of 'marker' genes involved in various processes in early bovine embryonic development. Transferable morulae and blastocysts produced in vitro expressed most genes similar to their in vivo counterparts. These data contribute to the molecular characterization of this widely used in vitro culture system for bovine embryos and provide a major advance towards production of 'physiologically normal' embryos.
本研究调查了半限定培养系统对参与致密化和空泡化的基因RNA表达时间模式的影响,这些基因包括:缝隙连接蛋白连接蛋白43(Cx43)、桥粒糖蛋白桥粒芯糖蛋白1(Dg 1)、桥粒胶蛋白I、II和III(Dc I、Dc II、Dc III)、桥粒蛋白斑联蛋白(Plako);代谢葡萄糖转运蛋白-1(Glut-1);RNA加工聚腺苷酸聚合酶(PolyA);热休克蛋白70.1(HSP);以及滋养层功能滋养层蛋白(TP),使用添加牛血清白蛋白的TCM199作为培养基体外生成牛卵母细胞和胚胎。从超排小母牛收集体内来源的桑葚胚和囊胚,并用于本研究。从20 - 50个卵母细胞或胚胎的样本中提取Poly(A)+ RNA,通过逆转录-聚合酶链反应进行分析,并通过测序验证扩增片段。每个发育阶段的测定至少重复三次,所有重复均得到一致结果。在体外产生的牛胚胎中,编码Cx43的mRNA在桑葚胚阶段之前均可检测到,而囊胚和孵化囊胚不表达该基因。在整个测试的着床前阶段均未发现Dg 1和Dc I的转录本。从2 - 4细胞胚胎到孵化囊胚阶段均可发现Dc II和Dc III的转录本。在未成熟和成熟卵母细胞以及合子中检测到编码Plako的mRNA,而在2 - 4细胞和8 - 16细胞胚胎中未见到转录本。该基因在桑葚胚到孵化囊胚阶段再次表达。体外产生的卵母细胞和牛胚胎在整个着床前发育直至孵化囊胚阶段均显示出Glut-1、PolyA和HSP的转录本。编码TP的基因仅在囊胚和孵化囊胚中被转录。体内产生的桑葚胚和囊胚与其体外对应物表现出相同的表达模式,但有一个例外:体内胚胎转录Cx43。本研究结果首次揭示了一组参与牛早期胚胎发育各种过程的“标记”基因的转录模式。体外产生的可移植桑葚胚和囊胚表达的大多数基因与其体内对应物相似。这些数据有助于对这种广泛用于牛胚胎的体外培养系统进行分子表征,并为生产“生理上正常”的胚胎提供了重大进展。
