Molecular Phylogeny of Slow Lorises (Nycticebus) Revealed by D-loop Sequences and Complete Cytochrome b Gene Sequences of Mitochondrial DNA

Partial sequences of the D-loop and the complete sequences of cytochrome b gene (1 140 bp) of the slow lorises (genus Nycticebus) were undertaken to investigate evolutionary relationships among species of Nycticebus.Sequence analysis results consistently provide new taxonomy evidence at the DNA level for supporting Ratajszczak and Groves’ viewpoint that N.intermedus is merely the adult of N.pygmaeus (Ratajszczak,1998;Groves,1971).Phylogenetic analysis was performed by means of the combined data and these two separate sequences data,respectively,by using various methods,supporting the same topology,in which genus Nycticebus was formed of two clusters.The first cluster was composed of N.pygmaeus,and the second cluster of N.coucang.It also could provide a new molecular genetic evidence to support the view that the genus comprises two species:N.coucang and N.pygmaeus.

Mutations of mitochondrion DNA in mouse tumors

Objective： To ascertain the variations of mitochondrion DNA （mtDNA） in mouse tumors and to inquire into the relationship between mutations of mtDNA and carcinogenesis Methods： The variations of D-loop, ND3 and tRNA^Met＋Glu＋Ile gene fragments of mtDNA from six tumor cell lines of mice were analyzed by PCR technology with restriction fragment length polymorphism analysis （polymerase chain reaction-restriction fragment length polymorphism, PCR-RFLP） and single strand conformation polymorphism analysis （SSCP-PCR） method. Results： ND3 and tRNA^Met＋Glu＋Ile gene fragments ofmtDNA from the tumors showed no variation in 27 endonuclease sites; D-loop ofmtDNA from Hca-F had an additional endonuclease sites of Hinf I in contrast to that of the inbred mouse. Deeply analyzed by PCR-SSCP, the D-loop ofmtDNA was found to possess mutations in 4 of 6 tumors. Conclusion： D-loop is the hot spot of tumor mtDNA mutation which can act as contributors to the carcinogenic

线粒体DNA数目不同的人角质形成细胞模型的建立

该研究采用溴化乙锭(ethidium bromide,Et Br)对人永生化角质形成细胞(HaCaT)进行诱导,采用RT-PCR法、MTT法和健那绿染色技术联合鉴定Et Br对HaCaT细胞线粒体DNA(mitochondrial DNA,mt DNA)拷贝数的影响,建立不同mt DNA拷贝数目的HaCaT细胞模型。结果显示,HaCaT细胞经100 ng/m L和50 ng/m L Et Br分别处理10 d后,细胞形态随着处理时间的延长发生改变,由规则铺路石形状逐渐变圆,某些细胞体积变小,成团生长,细胞膜边缘不光滑,且随着mt DNA数目的减少,细胞增殖速率明显下降。RT-PCR分析结果显示,与对照组相比,50 ng/m L和100 ng/m L Et Br处理10 d的HaCaT细胞中,mt DNA的拷贝数分别减少了52.9%和97.6%[以线粒体DNA脱氢酶1(mitochondrial NADH dehydrogenase 1 gene,ND1)与甘油醛-3-磷酸脱氢酶(glyceraldehyde-3-phosphate dehydrogenase,GAPDH)的比值来表示mt DNA的相对拷贝数变化情况]。健那绿染色显示,对照组HaCaT细胞中可见分散存在的蓝绿色线粒体颗粒,100 ng/m L Et Br处理10 d后的HaCaT细胞中,显微镜下蓝绿色线粒体颗粒明显减少。综上所述,该研究证明了HaCaT细胞可通过Et Br诱导被成功培养成ρ–细胞,且Et Br浓度与HaCaT细胞mt DNA拷贝数的变化在一定的范围内存在着剂量–效应关系。

小鼠DNA双链断裂修复缺陷细胞的γ射线剂量率效应

目的 探讨γ射线照射后小鼠DNA双链断裂修复缺陷细胞 (SCID)的剂量率效应和潜在致死性损伤的修复。方法 采用低剂量率和高剂量率以及间隔 2 4h的 2次γ射线照射正常细胞(CB .17+/ +)和SCID细胞 ,通过成克隆分析法观察被照射细胞的存活分数。结果 应用间隔 2 4h的2次γ射线照射CB .17+/ +细胞时 ,其存活分数明显高于相同剂量的单次照射 ,而SCID细胞二者无明显差异。在高剂量率单次和 2次γ射线照射时 ,SCID细胞均比CB .17+/ +细胞更敏感。在低剂量率γ射线照射时 ,SCID细胞亦显示比CB .17+/ +细胞更敏感。低剂量率γ射线照射CB .17+/ +细胞和SCID细胞后 ,二者的存活分数均明显高于高剂量率照射。结论 SCID细胞不具有DNA双链断裂的修复能力。SCID细胞和CB .17+/ +细胞均具有剂量率效应。

Phylogeny of Apaturinae Butterflies (Lepidoptera: Nymphalidae) Based on Mitochondrial Cytochrome OxidaseⅠ Gene

The phylogenetic relationships of genera in the subfamily Apaturinae were examined using mtDNA sequence data from 1,471 bp of cytochrome oxidase subunit Ⅰ （COI）. The mitochondrial COI gene from a total of 16 species in 11 genera were sequenced to obtain mtDNA data, along with those of 4 species obtained from GenBank, to construct the MP and the NJ trees using Athyma jina, Penthema adelma, Polyura nepenthes, and Charaxes bernardus as outgroups. The transitions at the third codon positions of the COI data set were found saturated, but they were retained for analysis, because they contain the majority of the phylogenetic information. The impacts of equal weight assumptions for all characters in the parsimonious analysis were assessed by potential alternations in clades in response to different transition/transversion weighting schemes. The results indicated four distinct major groups in Apaturinae. Moreover, several well supported and stable clades were found in the Apaturinae. The study also identified undetermined taxon groups whose positions were weakly supported and were subject to changes under different weighting schemes. Within the Apaturinae, the clustering results are approximately identical to the classical morphological classification. The mtDNA data suggest the genus Mimathyma as a monophyletic group. Lelecella limenitoides and Dilipa fenestra have close relationship with very strong support in all phylogenetic trees. It also supports the taxonomic revision of removing several species from Apatura to other genera, namely Mimathyma schrenckii, M. chevana, M. nycteis, Chitoria subcaerulea, C. fasciola, C. pallas, and Helcyra subalba.

Genotypic Assessment by RAPD Markers and Ultrastructural Characteristics of a NaCI-Tolerant Potato Cell Line

Salinity is a serious threat to agricultural production. Potato （Solanum tuberosum） is an important food crop characterised for having low to moderate salinity tolerance. Tissue cultures may be relevant to improve salt tolerance in potato through selection of salt-tolerant cell lines and subsequent regeneration of plants. In this work, the authors used the random amplified polymorphic DNA （RAPD） markers to investigate the occurrence of genetic polymorphism in a potato calli line tolerant to 150 mM NaCI. Out of 40 primers screened, eight generated polymorphic patterns that distinguished salt-tolerant line from the control. Although the macroscopic appearance was similar in both lines, ultrastructural study revealed alterations in salt-grown cells. These showed that plastids less differentiated with a lower number of grana had more and larger starch grains than control cells. In conclusion, RAPD analysis revealed that NaCl-adapted line is a somaclonal variant and the ultrastructural study showed changes essentially at the plastids.