花生胚小叶体细胞植株再生系统的建立

[目的]研究花生胚小叶体细胞植株再生体系,为利用胚小叶进行外源基因遗传转化提供试验依据。[方法]以花生品种四粒红和改良海花的胚小叶为外植体,2种外植体取材方式(预培养和直接取材)为培养背景,探讨了不同取材方式下各个培养要素(基因型、培养基等)与脱分化、再分化的关系,初步建立了花生胚小叶体细胞植株再生体系。[结果]在预培养取材条件下,预培养6d的四粒红外植体在2号培养基(MS+3mg/L6-BA+1mg/LNAA)上分化得最好,每愈伤组织再生芽2.34个,预培养5d的改良海花外植体在1号培养基(MS+5mg/L6-BA+3mg/LNAA)上分化最佳,每愈伤组织再生芽2.08个。直接取材条件下,改良海花在1号培养基上每愈伤组织出芽数为6个,而四粒红为3个。直接取材在诱导愈伤组织及器官分化方面都好于预培养取材。[结论]直接取材条件下,不同培养基对诱导愈伤组织及芽分化的作用差异较大,而基因型在诱导愈伤组织上的作用有显著差异,在出芽率上的作用差异并不显著。     

棉花耐盐胚性细胞系筛选及其植株再生

 继代1年以上的棉花品种珂字201下胚轴产生的胚性愈伤组织，转入加有不同浓度[0、8.56×10#+(-2)、1.71×10#+(-1)、2.57×10#+(-1)、3.42×10#+(-1)、5.13×10#+（-1）、6.84×10#+（-1）mol/L]NaCl的筛选培养基上培养，经过3代筛选，获得耐盐胚性细胞系和再生植株。NaCl显著抑制了愈伤组织的存活和生长，NaCl半致死浓度在8.56×10#+（-2）～1.71×10#+（-1）mol/L之间，致死浓度为6.84×10#+（-1）mol/L。NaCl浓度影响着体细胞胚的发生和发育，影响着体细胞胚的萌发和植株再生。添加1.71×10#+（-1）mol/L NaCl培养基，筛选出的愈伤组织生长较好，并能分化出体细胞胚和正常再生植株。在本实验中，笔者获得了耐3.42×10#+（-1）mol/L NaCl的体细胞胚和耐1.71×10#+（-1）mol/L NaCl的正常再生植株。     

JYG-1型移动喷灌机的研制

在广泛调研的基础上,开发出了适合温室使用的JYG-1型移动喷灌机。该型喷灌机主要由供水系统、行走系统、电气控制系统三大部分组成,综合采用了编程控制、变频调速、无线电遥控等技术,具有使用方便、自动化程度高、喷洒均匀度高等显著特点,并已在全国各地推广应用。     

Research on Isolation and Clone of Embryonic Stem Cell-Like in Bovine

Bovine embryonic stem cell would be invaluable for researching the aspect of animal cloning, production transgenic animal and discussion of gene function in vitro. With the object of establishing an effective culture system for isolation and clone of bovine pluripotent stem cell, we cultured bovine embryos and mouse embryos including morula blastula and hatached blastula and obtained animal ICM on Primary marine embryonic fibroblast (Primary murine embryonic fibroblast, PMEF) feeder layer with tissue medium(DMEM supplemented with 15ml/100ml NBS ,0.1μmol/L Na2SeO3, 0. 1mmol/L β-mercaptoethanol, 1 000ng/ml LIF,10 ng/ml IGF, 1mmol/L necessary amino acid and 1mmol/L L-glutamine), then, we obtained mouse ICM and bovine ICM. Moreover, we isolated and cloned the 6 passage bovine ES like cells(12 cell lines) and 9 passage marine ES like cells (52 cell lines) deriving from bovine ICM and murine ICM respectively on the feeder layer of PMEF by disaggregating ICM and ES cell clones of bovine and murine into smaller clumps through digesting with 0. 125g/100ml trypsin and 0.02g/100ml EDTA and scattering with a glass needle. The pluripotency of both murine and bovine ES like cells was identified with morphological character, histochemistry identification, karyotype analysis and differentiation of ES cells in vitro or in vivo. This result showed that bovine embryonic stem cell and murine embryonic stem cell had developmental pluripotency.     

支持牛类胚胎干细胞发育的饲养层培养体系的建立

以小鼠胎儿和牛睾丸为材料 ,以含 1 5 % NBS、0 .1 mmol/ Lβ-巯基乙醇、0 .1 μmol/ L Na2 Se O3的DMEM溶液为培养液 ,分离获得了传 1 5代的小鼠胎儿成纤维细胞和 5代牛睾丸成纤维细胞 ,建立了小鼠和牛类 ES细胞培养体系。结果表明 :牛睾丸成纤维细胞和小鼠胎儿成纤维细胞均属附着生长型细胞 ,与小鼠胎儿成纤维细胞相比较 ,牛成纤维细胞直径和长度大 ,生长速度快 ,易于老化 ;1 2～ 1 6日龄的小鼠胎儿最适宜分离与克隆小鼠胎儿成纤维细胞 ;在 2 5℃条件下 ,以 0 .2 5 %胰蛋白酶 0 .0 4% EDTA消化液作用胎儿小块组织分离原代小鼠胎儿成纤维细胞 ,消化液作用时间不应超过 2 0 min,以相同的消化液在 3 7℃条件下 ,离散贴壁成纤维细胞 ,作用时间以 2～ 3 min为宜 ;培养细胞密度与传代时间间隔有密切关系 ,若传代时间间隔为 3～ 4d,培养细胞浓度应为 3× 1 0 5个 / ml～ 5× 1 0 5个 / ml;在成纤维细胞分离与克隆过程中 ,培养基中添加0 .1μmol/ L Na2 Se O3 0 .1 mmol/ Lβ-巯基乙醇 1 5 % NBS,有利于 MEF和 NBTF的增殖     

Metanephric cell microenvironment induces embryonic stem cells to differentiate toward renal cells

AIM: To explore the effects of metanephric cell microenvironment on inducing embryonic stem cells (ESCs) to differentiate toward renal cells.METHODS: Embryoid bodies (EBs) of D3 mouse embryonic stem cells were prepared by hanging drop culture, and the EBs were co-cultured indirectly with metanephric cells derived from E12.5 d mouse embryo. The EBs cell with spontaneous differentiation was used as the control. The proteins of Pax2 and WT-1 were analyzed by immunofluorescence assay. The mRNA expression of Pax2, WT-1, Lim1, Sall1, Emx2, GDNF, Wnt4, BMP7, Nephl, Nephrin, KSP and CD24 genes was detected by RT- PCR.RESULTS: The genes related to kidney development were expressed in the EBs cells after co-culture on day 3, and the mRNA expression of Pax2, WT-1, Emx2, GDNF, Nephl, Nephrin, KSP and CD24 was stronger than those in control group. Pax2 positive cells were found on day 3 in the co-cultured EBs cells, and the positive cells increased on day 5 and day 7. WT-1 protein positive cells were found in the co-cultured EBs cells on day 5. No Pax2 or WT-1 positive cell was observed in control group.CONCLUSION: Metanephric cell microenvironment promotes ESCs differentiation toward renal cells.     

Supportive effects of human AGM region and fetal liver stromal cells on differentiation of murine embryonic stem cells into hematopoietic stem cells and in vivo hematopoietic reconstitution

AIM: To investigate the differentiation of murine embryonic stem cells (ESCs) into hematopoietic stem cells (HSCs) by the supportive effects of human aorta-gonad-mesonephros (AGM) region and fetal liver (FL) stromal cells.METHODS: E14 ESCs were induced into embryoid body (EB) first. Then the cells from EB were further co-cultured with human AGM region and FL stromal cells in non-contact system. On day 6, the cells derived from EB were collected for Sca-1⁺c-Kit⁺ cell analysis by flow cytometry, colony forming unit (CFU) assay and teratoma formation checking. BALB/c female mice conditioned with lethal dose of γ-ray irradiation were transplanted with EB cells from different culture systems. The survival rates, engraftment of donor cells, reconstitution of hematopoietic were monitored.RESULTS: Sca-1⁺c-Kit⁺ cells in EB cells co-cultured with human AGM region and FL stromal cells had the value of (21.96±2.54)%, and the total CFU was as (520±52)/10⁵ cells, which were statistically greater than those in EB cells only cultured with human AGM region stromal cells (P＜0.05). No teratoma was found in NOD-SCID mice after subcutaneous injection of EB cells co-cultured with human AGM region and FL stromal cells. In BALB/c female mice transplanted of EB cells co-cultured with human AGM region and FL stromal cells, the survival rate was 77.8%, and the peripheral blood cell count was obviously improved on day 14. PCR results showed the recipients all had sry gene copies from donor in bone marrow. The recipient mice transplanted with EB cells only cultured with human AGM region stromal cells all died within 15 days.CONCLUSION: Stromal cells from human AGM region and FL enhance the directed differentiation of ESCs into HSCs which can reconstruct hematopoiesis in vivo.     

锦橙果实发育过程中香气成分的变化

为了研究锦橙果实发育过程中香气成分的组成及变化,使用气相色谱-质谱联用仪分析了10月、11月、12月、翌年1月的锦橙鲜果的挥发性成分,分别检测到47,50,57,46种成分,主要成分为烃类、醛类、醇类和酯类.挥发性物质的总峰面积以及烃类、酯类在12月的果实中达到最大,反式-2-己烯醛、反式-2-己烯-1-醇、顺式-3-...     

Low reproductive success of leatherback turtles, Dermochelys coriacea, is due to high embryonic mortality

We examined the mechanism responsible for low reproductive success in leatherback turtles (Dermochelys coriacea) at Playa Grande, Costa Rica: low egg fertilization versus high rates of embryonic death. Leatherbacks at this beach had a high rate of fertility (=93.3%±2.5%, n=819). We incubated 10 eggs from every clutch encountered of 19 females during 3 months of the 1998-1999 nesting season. Fertility rate of some females decreased during the nesting season, but overall was high. Detection of fertility was difficult using standard methods because fertility rates cannot be determined accurately from nests excavated after hatching because of egg decomposition. Removal and incubation of eggs from nests provided a better estimate. Embryonic death, particularly in the beginning of incubation before embryos are visible to the unaided eye, was the cause of low hatching success in this population. Hatching success increased with increasing fertility and differed between females, with some mothers having 71-81% success and others 23-32%. Embryonic death and not low egg fertility drives poor recruitment at Playa Grande. Improved conservation of this species at Playa Grande will require a better understanding of the mechanism behind embryonic death.     

鹅肌球蛋白重链1基因MyHC1全长cDNA克隆、序列及胚胎期表达特征分析

肌球蛋白是组成肌原纤维粗丝的主要成分,在肌肉生长发育和运动收缩过程起重要作用。本研究采用反转录PCR和快速扩增cDNA末端(rapid amplification cDNA ends,RACE)方法,从太湖鹅(Anser anser)肌肉中克隆到肌球蛋白重链1基因(myosin heavy chain 1,MyHC1)的全长cDNA,并运用生物信息学的方法对其进行分析,实时荧光定量PCR(Real-time fluorescent quantitative PCR,qRT-PCR)检测MyHC1基因在鹅胚胎期的表达情况。研究结果表明,鹅MyHC1基因(Gen Bank登录号:KM675469)cDNA全长6028 bp,包含5 823 bp的开放性阅读框,57 bp的5’端非编码区和148 bp的3’端非编码区,共编码1 940个氨基酸。经预测,鹅MyHC1基因编码的蛋白质由31 478个原子组成,分子式为C9746H15817N2753O3096S66,相对分子质量为223 kD,等电点为5.62,平均亲水性为-0.786,属于不稳定亲水蛋白。在线预测鹅和鸡(Gallus gallus)的MyHC1蛋白质三维结构呈高度相似,由多螺旋和折叠片聚集成球状头部,并带有长纤维状α-螺旋尾部。鹅MyHC1的编码区(coding sequence,CDS)序列与鸡的同源性最高,为92.86%,与哺乳类同源性多数在84%左右,与两栖类同源性相对较低。鹅与鸡氨基酸同源性最高,为96.45%,与哺乳类的同源性多数在90%左右,与非洲爪蛙(Xenopus laevis)同源性较低,为78.13%。系统进化树分析表明,哺乳动物形成一个大分支,两栖类自成一支,鹅和红原鸡聚成一支,分子进化地位的关系最近,验证了鹅和鸡属于近缘物种。qRT-PCR检测到MyHC1基因在胚胎期第7天开始表达,以后表达量逐渐升高,在15d表达量达到高峰后下降,25d之后逐渐趋于平稳,表明,MyHC1基因在鹅胚胎期mRNA水平的表达量呈先上升再下降的趋势。本研究首次获得了鹅MyHC1的全长cDNA序列、分子的结构特点和表达特征,显示该基因在鹅肌肉生长发育过程起重要作用,为该基因的功能及鹅肉质性状研究提供了基础资料。