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1.
刺槐宽叶和四倍体无性系的组织培养   总被引:13,自引:0,他引:13  
1植物名称刺槐(Robiniapseudoacacia)优良无性系:Tetraploidlocust、Glgastypelocust。2材料类别带腋芽的茎段。3培养条件(1)启动培养基:MS+6-BA0.25mg·L-1(单位下同)+NAA0.05。(2)分化培养基和继代培养基:MS+6-BA0.5+NAA0.1+AgNO310,MS+6BA0.5+NAA0.1。上述培养基均添加3%蔗糖、0.6%琼脂。(3)生根培养基:1/2MS+IBA0.2+NAA0.2,添加2%蔗糖0.6%琼脂。培养基pH…  相似文献   

2.
几种鲟鱼基因组大小、倍体的特性及鲟形目细胞进化的探讨   总被引:27,自引:2,他引:25  
采用Feulgen-显微分光光度计方法,以鸡红细胞为标准DNA(3.22pg/2C)测定了长江白鲟、达氏鲟、中华鲟、史氏鲟和北美匙吻鲟的体细胞基因组大小(DNA含量)。结果表明,上述五种鲟鱼DNA含量分别为4.11、8.26、9.07、6.07和3.96pg。长江白鲟和北美匙吻鲟均属于四倍体鱼类,分布在长江水系的中华鲟和达氏鲟两种鲟属鱼类为八倍体类型。史氏鲟初步判断为八倍体,据分析可能存在四倍体的  相似文献   

3.
氧化诱导K_(562)细胞凋亡机制的初步探讨   总被引:7,自引:0,他引:7  
以过氧化氢(H2O2)诱导人慢性髓细胞白血病(K562)细胞为凋亡模型,采用流式细胞仪(flowcytometry,FCM)和激光共聚焦扫描显微镜(laserconfocalscanningmicroscopy,LCSM)研究细胞凋亡,形态观察出现核固缩,核碎裂及凋亡小体等典型凋亡特征.DNA电泳图谱出现“Ladder”.FCM检测在G0/G1峰前出现一低DNA含量的凋亡峰.LCSM显示凋亡细胞c-Fos.c-Jun和NFκB表达量均有不同程度的增加.该结果提示上述三种转录因子可能参与氧化诱导凋亡过程中基因的调控作用.  相似文献   

4.
利用微丝(microfilament,MF)解聚药物细胞松驰素B(cytochalasinB,CB)处理G_0期小鼠C_3H_(10)T_(1/2)成纤维细胞,对G_0至S期DNA合成,胸腺嘧啶核苷激酶(thymidinekinase,TK)活性、TK基因表达、钙调素(calmodulin,CaM)水平和一些细胞周期早期基因的表达进行了观察,G_0期细胞经3mg/LCB处理2h,促MF解聚增强了血清对S期细胞TK活性、TK基因表达和DNA合成的刺激作用,并促进细胞提前进入S期.血清刺激G_0期细胞进入晚G_1期和S期时,CaM水平明显升高,而CB预处理则使CaM含量进一步增加,特别是CB处理促使S期CaM增加向核内转移.CB处理明显增强血清对c-jun、c-fos和c-myc基因表达的刺激作用,而PKC抑制剂H_7则抑制CB处理对这些基因转录的刺激作用,说明CB使G_0期细胞MF解聚刺激c-jun、c-fos和c-myc的转录活性与PKC的作用有关.结果表明G_0至S期早期MF的重组可促进细胞进入S期,增强DNA合成.  相似文献   

5.
ELISA技术筛选200种中草药抗HBsAg的实验研究   总被引:9,自引:0,他引:9  
使用ELISA技术对200种中草药水提取物进行抗HBsAg的实验研究,共筛出有效药物7种(占总数的3.5%)。若按5种不同剂量(0.3、0.6、1.2、2.5、5.0mg/100μl)的药物、2种不同浓度的HBsAg(10.92、14.26P/N值)与3种不同接触时间(立即、1h、2h)的10项P/N值均数来综合评价药效指数时,7种有效药物的次序为青蒿(1.67P/N值)、大蒜(2.19P/N值)、红孩儿(2.31P/N值)、仙鹤草(2.31)、魔芋(2.32P/N值)、冬瓜皮(2.63P/N值)和猕猴桃(2.89P/N值)。  相似文献   

6.
用流式细胞光度术(floweytometry,FCM)+S0.2ml/日。吐温对照组lP吐温800.2ml/日,以排除大蒜油制剂中溶剂(吐温80)的影响。实验组lPGO100mg/kg/.日。于连续4次注射后的6h,2、3、5、10天及10次注射GO后7天取材,行FCM样品制备。三、FCM样品制备与测定中国中医研究院基础所腹水癌细胞用PBS洗涤,70%酒精固定,RNase消化细胞中的RNA,PI染色。用腹腔内淋巴细胞作标准二倍体细胞。用420型荧光激活细胞分选仪(美国Becto-Dickson公司产品)测单个肿瘤细胞的DNA含量,用组方图显示肿瘤细胞DNA倍体性质。图中第一个是DNA二倍体(ZC)峰,处于该峰的细胞为G;/G。期细胞,第二个峰为4CDNA峰,该处细胞为G。-I--M期细胞,从2。到4。之间的细胞为S期细胞。大于4。DNA峰细胞为高倍体细胞‘’:。根据不同峰值大小判定用药后肿瘤细胞倍体性质的变化。结果NS与吐温对照组肿瘤细胞都为非整倍体性,且呈多倍体性(图1,2)。连续4次给药后6h,绝大部分多倍体肿瘤细胞被杀伤,残存肿瘤细胞以二倍体为主,多倍体肿瘤细胞峰值显著下降,甚至在组方图上几乎显不出多倍  相似文献   

7.
在无血清和含1.0%、5.0%血清培养的新生大鼠心肌细胞标本上,去甲肾上腺素(NE,2.0μmo1/L)使细胞蛋白质含量(Lowry法)分别比相应对照组增加40%、26%、19%(P均<0.01);细胞^3H-亮氨酸参入量与NE浓度呈正性剂量依赖性,最大效应浓度为20.0μmo1/L;无血清培养体系中,0.2.2.0、20μmo1/L的NEW使参入量分别比对照增加17.8%、35.3%、37.7%  相似文献   

8.
NNK诱发BEP2D细胞产生活性氧及其对DNA的损伤   总被引:4,自引:0,他引:4  
通过测定细胞内和细胞上清中活性氧(reactive oxygen species,ROS)水平,以及DNA 加合物——8-羟基脱氧鸟嘌呤核苷(8-hydroxydeoxyguanosine,OH8dG)含量,对烟草特异亚硝胺类化合物4-甲基亚硝胺-1(3-吡啶基)-1-丁酮(4-(m ethylnitrosam ino)-1-(3-pyridyl)-1-butanone,NNK)诱发人乳头状病毒永生化的人支气管上皮细胞(hum an papillom avirus-im m ortalized hum anbronchialepithelialcellline,BEP2D)产生的ROS及其对DNA 的氧化损伤进行研究,并观察纳米硒的保护作用.结果表明,BEP2D 细胞经不同浓度的NNK 作用后,细胞内和细胞上清中ROS以及OH8dG含量均显著增加,并有较好的剂量效应关系.1 μm ol·L- 1纳米硒(nanoselenuim ,NS)能明显抑制NNK 诱发BEP2D细胞产生的ROS及OH8dG 水平.揭示NNK 能造成细胞的氧化损伤,而NS对NNK 所致细胞的氧化损伤有保护作用.  相似文献   

9.
克隆小鼠白细胞介素12(IL-12)p40及p35cDNA,并构建同时含mIL-12p40和p35cDNA的双顺反子真核表达载体及其在哺乳动物细胞中的表达.白细胞介素12是由巨噬细胞,树突状细胞等抗原提呈细胞产生的一种异二聚体细胞因子,对机体的细胞免疫功能起着重要的调节作用.利用脂多糖(100pg/ml)和小鼠重组干扰素(IFN-γ500U/ml)体外联合刺激小鼠腹腔巨噬细胞,从中提取总RNA,经RT-PCR扩增出含信号肽的小鼠白细胞介素12(mIL-12)p40及p35全长cD-NA.PCR产物经酶切后,分别克隆至pBluescriptⅡSK载体中,序列测定结果与文献报道序列一致.然后利用脊髓灰质炎(Polio)病毒内核糖体进入位点(IRES)连接mIL-12p40及p35cDNA,亚克隆至pcDNA3载体中,构建成含mIL-12p40及p35cDNA双顺反子真核表达载体,即pcDNA3/mIL-12,p40及p35cDNA同时受pcDNA3中hCMV启动子驱动,将p40及p35转录至同一mR-NA上.通过LipofectAMINE将pcDNA3/mIL-12转染COS-7细胞,72h收集培养上清,测定m  相似文献   

10.
脂多糖对离体培养大鼠血管平滑肌细胞增殖的影响   总被引:2,自引:0,他引:2  
Li J  Lin SX  Li Y  Zhao HL  Jia B 《生理学报》1999,51(1):14-18
本研究观察到10-7~10-5kg/L脂多糖(lipopolysacharide,LPS)可显著促进血管平滑肌细胞(VSMC)的增殖及DNA的合成(P<005)。5×10-4~10-3kg/LLPS却抑制VSMC的增殖及DNA的合成,降低其活力(P<001),并呈时间依赖效应。一氧化氮合酶抑制剂NNitroLArginine(LNNA)可拮抗LPS的抑制作用。大剂量LPS作用组VSMC上清液中一氧化氮(NO)代谢产物NO-3和NO-2的含量与对照组相比显著增加(P<001),48h组比24h组增加91%,72h组比48h组增加45%;同时,诱导性一氧化氮合酶(inductivenitricoxidesynthase,iNOS)免疫组化染色呈阳性。结果表明,低浓度LPS促进VSMC增殖和DNA合成,而高浓度LPS却明显抑制VSMC增殖和DNA合成,降低其活力。这种抑制作用可能与LPS诱导VSMC产生的NO有关。  相似文献   

11.
Flow cytometric DNA analysis was used to determine the DNA content of red blood cells from Ginglymostoma cirratum (Bonaterre) and Raja eglanteria (Bosc). The DNA content/nucleus was calculated to be 7.6 and 7.1 pg/nucleus, respectively. Peripheral red blood cells obtained both from G. cirratum and from R. eglanteria were demonstrated to be actively cell cycling. Percentages of red blood cells in the phases of the cell cycle ( G 0/ G 1, S , and G 2/ M ) not only varied considerably between different fishes but also were quite variable in weekly samples obtained from individual animals.  相似文献   

12.
黄喉拟水龟细胞核DNA含量的分析   总被引:10,自引:0,他引:10  
以黄喉拟水龟 (Mauremysmutica)的红血细胞为材料 ,以鸡红血细胞为DNA标准 ( 2 5pg/2c) ,采用流式细胞仪测定了黄喉拟水龟及其两个种群的细胞核基因组DNA含量。黄喉拟水龟的细胞基因组DNA含量为 5 16± 0 2 9pg/2c (n =6 0 ) ;南方种群的细胞核DNA含量为 5 19± 0 30pg/2c (n =30 ) ,北方种群为 5 14±0 30pg/2c (n =30 ) ,两个种群的核DNA含量无显著差异 (t=0 6 84 7,df =5 8,P >0 0 5 )。  相似文献   

13.
A J Walle  G Y Wong 《Cytometry》1988,9(2):170-176
In 47 healthy blood donors (controls) and 29 renal allograft recipients (patients) the relative contents of RNA and DNA of peripheral blood mononuclear (PBM) cell populations were estimated from the intensities of green and red fluorescences emitted by complexes that form with DNA and RNA, respectively, after staining the cells with the metachromatic dye, acridine orange. Based on the correlated DNA and RNA estimates for large numbers of cells, the percentages and the relative RNA contents of cells in particular compartments of the cell cycle were determined. PBM cell populations of controls contained less than 0.5% proliferating (SG2M) cells with highly variable relative RNA contents. Among controls, neither percentages nor relative RNA contents of SG2M-cells were correlated with percentages or relative RNA contents of G1-cells with an RNA content 2 (2SD) or 3 (3SD) standard deviations above the mean of the entire G0/1-cell population. Unlike controls, PBM cell populations of patients contained significantly higher percentages of SG2M-cells which were significantly correlated with the relative coefficients of variation (rCV) of the F530 histograms of G0/1-cells; the rCV represents the ratio of a patient's CV to a control's CV. Moreover, significant statistical correlations existed between percentages and relative RNA contents of 2SD-, 3SD-, SG2M- and G0/1-cells, suggesting a well-orchestrated progression of cells through the cell cycle. Different pairs of correlated parameters characterized clinically stable, acutely rejecting, and infected patients.(ABSTRACT TRUNCATED AT 250 WORDS)  相似文献   

14.
This report characterizes for the first time an easy, reproducible means of standardizing the relative fluorescent units normally reported for flow microfluorometry. Absolute values for deoxyribonucleic acid/cell are obtained by using nucleated red blood cells as references. Cell were selected and characterized for the quantitative analysis of deoxyribonucleic acid per cell over a range from 2 pg/cell to 93 pg/cell using literature values for species having nucleated erythrocytes. Fluorescence staining by either acridine-orange (green wavelength) or propidium iodide (red wavelength) gave linear curves over the entire range investigated only when "gain controls" and current are optimized. The range was equivalent to mammalian cell values from 1 N (=3.5 pg deoxyribonucleic acid/cell) to 28 N (=91 pg deoxyribonucleic acid/cell). The standard curves obtained with nonmammalian erythrocytes were compared to mammalian free-cell preparations of bovine thymus and liver cells which fell at 6.8 and 6.9 pg deoxyribonucleic acid/cell, respectively. The routine use of these easily obtainable red blood cells will allow ready comparisons on the basis of absolute values for deoxyribonucleic acid per cell for work between experiments, work between staining procedures and dye types and work between laboratories.  相似文献   

15.
Summary Differential staining patterns on amphibian chromosomes are in some respects distinct from those on mammalian chromosomes; C-bands are best obtained, whereas G- and Q-bands are either unobtainable (on anuran chromosomes) or coincide with C-bands (chromosomes of urodeles). In amphibians, rRNA genes are located at secondary constrictions, but in urodeles they are also found at other chromosome sites, the positions of these sites being strictly heritable. DNA content in amphibian cells is tens and hundreds times higher than in mammals. DNA contents in anurans and urodeles differ within certain limits: from 2 to 25 pg/N and from 30 to over 160 pg/N respectively. Species characterized by slow morphogenesis have larger genomes. Genome growth is normally due to an increase in the amount of repetitive DNA (mostly intermediate repetitive sequences), the amount of unique sequences being almost constant (11 pg/genome in urodeles, and 1.5 pg/genome in anurans). In anurans in general no satellite DNA was found, whereas such fractions were found in manyUrodela species. Nucleosome chromatin structure in amphibians is identical to that of other eukariotes. It is postulated that differences in chromosome banding between amphibians and mammals are due to differences in chromatin packing which in turn is related to the distinct organization of DNA repetitive sequences. It is likely that fish chromosomes have a similiar structure. A comparison of such properties as the chromosome banding patterns, variations in nuclear DNA content and some genome characteristics enable us to group fishes and amphibians together as regards chromosome structure, as distinct from amniotes - reptiles, birds and mammals. It is probable that in the ancient amphibians - ancestors of reptiles - chromatin packing underwent a radical transformation, following changes in the organization of DNA repetitive sequences.  相似文献   

16.
人们认为,细胞表面含碳水化合物的蛋白质可能在细胞相互作用中起着重要作用。从脊椎动物中分离出凝集因子以后(Teichberg et al., 1975;Nowak et al., 1977),许多研究表明这类凝集因子是与膜相结合的。这些发现支持了人们原先的设想。Beyer等人(1979;1980)从成体鸡肠中分离出一种结合乳糖的凝集因子,这种凝集因子似乎存在于粘液分泌小粒之中。1980年Pitts和Yang又从鸡胚肾脏中分离出一种结合乳糖的凝集因子,它可能是一种外周蛋白质。尽管他们的实验证明了成体鸡肾和肠这两种器官,同视网膜、肝脏、肌肉、心脏、脑和脊髓一样,存在着结合乳糖的凝集因子。但凝集因子在这两  相似文献   

17.
Rabbit antisera directed against an onco-developmental antigen on chicken red blood cells have been serologically dissected through specific adsorptions. It is now possible to detect 13 antigenic determinants with the fractionated antisera. The onco-developmental antigen referred to as chicken fetal-leukemic antigen (CFA) is fetal-specific in the white Leghorn chicken, being present on the embryonic but not adult peripheral red blood cells of non-being present on the embryonic but not adult peripheral red blood cells of non-leukemic birds. However, one or more of the onco-developmental antigenic determinants have been detected on adult peripheral red blood cells of non-Gallus avian species, as well as on red blood cells from two adult chicken varieties. For phylogenetic purposes, red blood cells from avian species were characterized for their combinations of CFA determinants. Comparisons among species revealed specific patterns of antigenic expression within phylogenetic groups. Several CFA determinants were restricted in their occurrence to species within a single family, and one determinant was found in all cases where CFA was expressed. The distribution of CFA determinants was used to determine immunological distances among four Galliform species. These distances agreed with the immunological relationships established using different serological markers.  相似文献   

18.
检测了37种中药对K562细胞生长及血红蛋白合成的影响,发现盐酸山莨菪碱(654-2)和三尖杉酯碱可以使K562细胞的血红蛋白细胞增加3倍,细胞平均血红蛋白含量增加4倍,γ珠蛋白mRNA的表达分别增加50%和40%。电泳结果显示HbF和γ珠蛋白肽链。  相似文献   

19.
1. Various blood indices in the Panamint kangaroo rat revealed seasonal fluctuations. The red blood cell count during winter and summer averaged 7.2 +/- 1.0 X 10(6) and 9.2 +/- 0.2 X 10(6)/mm3 respectively. 2. The mean cell hemoglobin during winter and summer averaged 25 +/- 10.8 pg and 18.6 +/- 3.7 pg respectively. 3. These fluctuations may reveal a rapid rate of red blood cell destruction during winter in combination with a change in diet, concomitant to this, is an increase in mean cell hemoglobin of the surviving red blood cells.  相似文献   

20.

Background

DNA repair is a cellular defence mechanism responding to DNA damage caused in large part by oxidative stress. There is a controversy with regard to the effect of red blood cells on DNA damage and cellular response.

Aim

To investigate the effect of red blood cells on H2O2-induced DNA damage and repair in human peripheral blood mononuclear cells.

Methods

DNA breaks were induced in peripheral blood mononuclear cells by H2O2 in the absence or presence of red blood cells, red blood cells hemolysate or hemoglobin. DNA repair was measured by 3H-thymidine uptake, % double-stranded DNA was measured by fluorometric assay of DNA unwinding. DNA damage was measured by the comet assay and by the detection of histone H2AX phosphorylation.

Results

Red blood cells and red blood cells hemolysate reduced DNA repair in a dose-dependent manner. Red blood cells hemolysate reduced % double-stranded DNA, DNA damage and phosphorylation of histone H2AX. Hemoglobin had the same effect as red blood cells hemolysate on % double-stranded DNA.

Conclusion

Red blood cells, via red blood cells hemolysate and hemoglobin, reduced the effect of oxidative stress on peripheral blood mononuclear cell DNA damage and phosphorylation of histone H2AX. Consequently, recruitment of DNA repair proteins diminished with reduction of DNA repair. This suggests that anemia predisposes to increased oxidative stress induced DNA damage, while a higher hemoglobin level provides protection against oxidative-stress-induced DNA damage.  相似文献   

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