Sequence of a Euplotes crassus Macronuclear DNA Molecule Encoding a Protein with Homology to a Rat Form-I Phosphoinositide-specific Phospholipase C

A 604-base pair macronuclear DNA molecule from the hypotrichous ciliate Euplotes crassus was cloned and its DNA sequence determined. The DNA sequence contains an open reading frame capable of encoding a protein 141 amino acids in length. The putative protein contains significant sequence similarity to other eukaryotic proteins, including the rat form-I phosphoinositide-specific phospholipase C.     

Micronuclear and Macronuclear Sequences of a Euplotes crassus Gene Encoding a Putative Nuclear Protein Kinase

The sequences of a 1.8-kbp macronuclear DNA molecule (V3), and the majority of its micronuclear counterpart, are reported. The macronuclear V3 DNA molecule contains an open reading frame that is interrupted by a single intron, while the micronuclear copy is interrupted by four internal eliminated sequences, one of which is located within the intron. The predicted protein product of the macronuclear V3 gene is a 471-amino acid polypeptide that is very similar to a group of protein-serine/threonine kinases from both plant and animal species, some of whose members appear to be involved in cell cycle or growth control.     

Conjugation-Specific Genes in the Ciliate Euplotes crassus: Gene Expression from the Old Macronucleus

ABSTRACT. Following mating or conjugation, the hypotrichous ciliate Euplotes crassus undergoes a massive genome reorganization process. While the nature of the rearrangement events has been well studied, little is known concerning proteins that carry out such processes. As a means of identifying such proteins, differential screening of a developmental cDNA library, as well as construction of a cDNA subtraction library, was used to isolate genes expressed only during sexual reproduction. Five different conjugation-specific genes have been identified that are maximally expressed early in conjugation, during the period of micronuclear meiosis, which is just prior to macronuclear development and the DNA rearrangement process. All five genes are retained in the mature macronucleus. Micronuclear, macronuclear, and cDNA clones of one gene ( conZ47 ) have been sequenced, and the results indicate that the gene encodes a putative DNA binding protein. In addition, the presence of an internal eliminated sequence in the micronuclear copy of the conZ47 gene indicates that this conjugation-specific gene is transcribed from the old macronucleus.     

蚕豆保卫细胞中ABA响应蛋白基因的转录

植物在不同的逆境条件下可以生成一类受脱落酸（ABA）诱导的蛋白质［脱落酸响应蛋白（ABAresPonsiveProtein，RABpr。tein）］（Bray1993）。RAB蛋白分布在不同的物种之中，许多［如Lea（Lateembryogen－。isabundant）蛋白（Dure1993）］形成于植物胚胎成熟失水过程中，但也有一些是植物受到不同逆境处理后在营养器官内所形成的「如脱水蛋白（Dehrdrin）］（Dure1993）。已发现的70余个RAB蛋白中，有30余个属于脱水蛋白。（Close等1993）RAB蛋白在植物体内的功能目前尚不了解（Bray1993）。由蛋白质的氨基酸组成分析表明，这些…     

Adolescence and the Reversibility of Maturity in Euplotes crassus

ABSTRACT. The clonal life history of ciliated protists is characterized by a sequence of phenotypes; sexual immaturity, maturity, and senescence. The distinctiveness of immaturity and maturity has been investigated. Standard assays of the onset of maturity of progeny clones from a cross between stocks EC1 and EC2 of Euplotes crassus demonstrated significant differences among clones and among testers within clones. They also revealed that the first positive test(s) of a progeny subclone were typically followed by at least one negative test. Special protocols were devised to investigate if maturity was reversible at the cellular level. In these experiments, the first mating pair of a progeny subclone was split before the consummation of mating. From these two cells as well as from control progeny and tester cells, subclones were established and every leftover cell was tested for maturity after each transfer. Both standard and split-pair progeny subclones had immature and slow- to-mate cells. The number of fissions before progeny exhibited sexual behavior indistinguishable from the testers was more than twice that to the first mating reaction of a subclone. At the first sign of maturity, progeny lines are a heterogeneous population of cells able and not able to mate, but remarkably, clonal descendants of those able to mate may become unable to mate. The development of maturity is progressive, quantitative and non-monotonic rather than an instantaneous switch.     

酵母内含子在基因序列中的分布对基因转录效率的影响

对酵母中高效转录和低效转录基因内含子序列寡核苷酸使用情况的对照分析,显示两类内含子的序列结构有差异,并且高效转录基因内含子序列含有较多潜在的转录因子结合位点,由此推测内含子可能参与基因转录的调控.这个结论有待更多的数据证实.对内含子和外显子在两组基因序列中的分布（长度、位置等）进行详细比较分析后显示,高效转录基因内含子和低效转录基因内含子的长度有比较明显的界限.两组基因中外显子长度的均值虽然有些差异,却没有明显的界限.基因序列长度与外显子长度的情况相似.虽然内含子的相对位置在两类基因中都很靠近5′端,但是从实际位置看,高效转录基因中比较多的内含子很靠近基因的5′端,有些则位于5′-UTR区域.这些结果提示,基因的转录效率与内含子的长度有关,与外显子及基因序列的长度无关,内含子的位置也可能影响转录效率,内含子对基因转录的调控可能与基因上游的转录调控有关联,或者是上游调控的延续.     

真核基因转录与转录调节相关复合物

真核细胞核中转录因子与染色质模板如何相互作用调节基因转录是基因表达调控研究的一个中心问题.近来的研究表明,参与基因转录的各种调节因子在核内形成多种复合物,如RNA聚合酶Ⅱ全酶、染色质重塑复合物、核小体以及增强小体等.这些复合物之间相互作用,调节染色质结构,在染色质模板上进一步组装成转录复合物,参与转录调节的各个环节,调节转录复合物活性.这些复合物的形成,整合了转录调节的各种信息,提高了转录调节效率,是真核基因有效、严格、有序表达的基础.另一方面,这些复合物的存在给基因表达调控的研究提出了新问题,发展新的研究思路和新的研究技术具有重要意义.     

亚硒酸钠对大鼠晶体蛋白基因转录的影响

对不同浓度的亚硒酸钠在体外对αA及β23晶体蛋白基因转录的影响作了初步的研究.结果发现,随着亚硒酸钠浓度的升高,αA基因的转录下降;而当亚硒酸钠浓度升至5×10^－5 mol/L时,αA基因的转录又呈反跳性回升;提示αA晶体蛋白在晶体细胞内,至少应答于高浓度的硒,可能作为一种应激蛋白表达.而随着硒浓度的增加,β23基因的转录则呈现出先升后降的双相变化;提示一定浓度的硒可能借某种机制影响或改变晶体上皮细胞的分化状态.     

Large scale synchronous mating and the study of macronuclear development in Euplotes crassus

After conjugation in hypotrichous ciliates, a new macronucleus is produced from a copy of the micronucleus. This transformation involves large-scale reorganization of DNA, with conversion of the chromosomal micronuclear genome into short, gene-sized DNA molecules in the macronucleus. To study directly the changes that occur during this process, we have developed techniques for synchronous mating of large populations of the hypotrichous ciliate Euplotes crassus. Electron microscope studies show that the micronuclear chromosomes are polytenized during the first 20 h of macronuclear development. The polytene chromosomes lack the band-interband organization observed in other hypotrichs and in the Diptera. Polytenization is followed by transectioning of the chromosomes. We isolated DNA at various times of macronuclear development and found that the average molecular weight of the DNA decreases at the time of chromosome transectioning. In addition, we have shown that a small size group of macronuclear DNA molecules (450-550 base pairs) is excised from the chromosomal DNA approximately 10 h later in macronuclear development.     

Differential DNA Amplification and Copy Number Control in the Hypotrichous Ciliate Euplotes crassus

ABSTRACT. During macronuclear development in hypotrichous ciliated protozoans, several thousand macronuclear DNA molecules are amplified several-hundred fold. We investigated the regulation of this amplification by determining the copy numbers of three different macronuclear DNA molecules in the hypotrichous ciliate Euplotes crassus. Two of the macronuclear DNA molecules were present in approximately 1,000 copies per cell, while the third was present in approximately 6,500 copies per cell. These reiteration levels were achieved either during macronuclear development, or shortly thereafter, and were maintained during vegetative growth. The most abundant macronuclear DNA molecule is present as a single-copy sequence in the micronuclear genome. Thus, its high copy number results from differential amplification. These results indicate that DNA amplification during macronuclear development is regulated individually for each macronuclear DNA molecule.     

肽链释放因子和核糖体蛋白L11在八肋游仆虫细胞中的定位

原生动物纤毛虫是一类单细胞真核生物,其蛋白质合成终止过程中密码子使用的特殊性使其成为研究蛋白质合成终止机制的一个经典模型。为了能够有效地分析生物大分子在该细胞中的功能作用位点,本研究根据该生物染色体结构的特征,构建了含有红色荧光蛋白基因的大核人工染色体EoMAC_R,并与之前构建的含绿色荧光蛋白基因的大核染色体EoMAC_G一起,对蛋白质合成终止有关的3个重要因子核糖体大亚基蛋白L11、多肽链释放因子eRF1和eRF3在八肋游仆虫细胞中进行了荧光共定位分析。结果显示,在八肋游仆虫细胞中,蛋白质翻译过程主要位于"C"形大核内侧区域。构建的人工染色体能够作为一种有效的工具,对目的蛋白质在八肋游仆虫细胞中进行定位分析。     

Morphology and SSU rDNA-based phylogeny of two Euplotes species from China: E. wuhanensis sp. n. and E. muscicola Kahl, 1932 (Ciliophora,Euplotida)

The living morphology, infraciliature and silverline system of two small Euplotes species, E. wuhanensis sp. n. and E. muscicola Kahl, 1932, isolated from Wuhan, central China, were investigated. Euplotes wuhanensis sp. n. is characterized by a combination of features including small size (40–50 × 25–30 μm), two conspicuously small and eight normal-sized frontoventral cirri, five transverse cirri in two groups, two marginal and two caudal cirri, seven dorsal kineties with about 12 dikinetids in the mid-dorsal row and a double-eurystomus type of dorsal silverline pattern. The Wuhan population of E. muscicola closely resembles previously described populations. The establishments of three subspecies of E. muscicola are not supported. The small subunit ribosomal RNA gene sequences were determined for both species. We propose that the two sequences under the name of E. muscicola (No. AJ305254, DQ917684 deposited in GenBank) are very likely from misidentified material. Phylogenetic analyses based on these data support the validity of both E. muscicola and E. wuhanensis as distinct species.     

休眠期和营养期包囊游仆虫的纤毛器骨架及其微管蛋白

应用光镜和透射电镜术 ,显示了包囊游仆虫休眠细胞中纤毛器骨架的形态 ,并对该纤毛虫休眠细胞和营养细胞的纤毛器及其α、β -微管蛋白进行了免疫荧光定位的比较研究。由免疫荧光显微术显示 ,包囊游仆虫形成休眠包囊后 ,背部毛基体完整地按原有模式保存下来 ;纤毛杆解聚后微管蛋白多集中在细胞皮层 ,小部分均匀散布在细胞质中。据所得结果认为 ,包囊游仆虫形成包囊后 ,微管蛋白主要有 3个去向 ,即 :①处于自噬泡内被逐步消化 ;②以“微管蛋白库”的形式分布于细胞皮层及细胞质中 ;③保留在残留的基体中。此外 ,以往研究中发现的棘毛基部纤维网络未被标记上 ,提示这些纤维体系可能不属于微管系统     

基因表达转录分析中内参基因的选择

目前基因表达的转录分析多采用单一看家基因作为内参来校正目标基因的表达量.实验中以人肝癌BEL-7402细胞为研究对象,应用实时荧光定量PCR技术,观察了新型三肽化合物酪丝缬肽作用后RPL13A、UBC、EIF4A、B2M、GAPDH和ACTB共6个看家基因mRNA水平的表达情况.经过geNorm程序统计学分析处理,结果表明,这6个看家基因的表达存在差异,确定了RPL13A、UBC2个看家基因用于校正目标基因的表达量.基因表达转录分析中内参基因选择的必要性在实验中得以证明,更重要的是为各种实验因素影响下(尤其是新物质作用下)内参基因的选择介绍和提供了一种行之有效的方法.