用TUNEL法检测植物原生质体的调亡

ＴＵＮＥＬ是近年来发展的一种凋亡细胞进行原位检测的方法,可以特异性地标记完整的凋亡细胞核或凋亡小体的染色体３’－ＯＨ断裂末端,但在植物细胞中的应用还不多。本文报道应用ＴＵＮＥＬ法检测胡萝卜原生质体的凋亡,并与ＤＮＡ电泳、彗星电泳等方法进行了比较,结果表明它是一种适用于植物原生质体凋亡检测的灵敏度较高的方法。     

细胞色素c能诱导植物细胞编程性死亡

以悬浮培养的胡萝卜（ＤａｕｃｕｓｃａｒｏｔａＬ．）与烟草（ＮｉｃｏｔｉａｎａｔａｂａｃｕｍＬ．ｃｖ．ＢＹ２）细胞原生质体为材料,加入一定浓度的细胞色素ｃ和ｄＡＴＰ。不同取样时间的ＤＡＰＩ荧光染色与电镜超薄切片观察的结果显示染色质发生凝集、趋边化,最终形成凋亡小体。核酸电泳显示ＤＮＡ发生特异降解并形成电泳“阶梯”（ＤＮＡｌａｄｄｅｒ）。用末端脱氧核糖核酸转移酶介导的ｄＵＴＰ切口末端标记方法（ＴＵＮＥＬ）检测发现ＤＮＡ的３＇ＯＨ断端被原位特异标记。以上结果说明：细胞色素ｃ能诱导植物细胞发生典型的凋亡。     

乙烯诱导胡萝卜原生质体凋亡

乙烯是一种参与多种重要生理学过程的植物激素。用乙烯利在密闭条件下处理胡萝卜（ＤａｕｃｕｓｃａｒｏｔａＬ．）原生质体（在ｐＨ＞４．１时释放乙烯）,发现随着乙烯利浓度增加,细胞死亡率逐渐增高。经乙烯利处理的胡萝卜原生质体出现核内染色质固缩,形成凋亡小体等典型的细胞凋亡的形态学特征。用中性法彗星电泳观测到彗星状的核ＤＮＡ片段的迁移。ＤＮＡ电泳分析观察到细胞凋亡时产生的典型的核小体间ＤＮＡ断裂所形成的梯状条带。结果表明,乙烯能诱导悬浮培养的胡萝卜原生质体凋亡     

用TUNEL法检测植物原生质体的凋亡

TUNEL是近年来发展的一种对凋亡细胞进行原位检测的方法,可以特异性地标记完整的凋亡细胞核或凋亡小体的染色体3'_OH断裂末端,但在植物细胞中的应用还不多。本文报道应用TUNEL法检测胡萝卜原生质体的凋亡,并与DNA电泳、彗星电泳等方法进行了比较,结果表明它是一种适用于植物原生质体凋亡检测的灵敏度较高的方法。     

药物诱导的玉米根尖凋亡细胞表面电特性研究(英文)

细胞凋亡过程中细胞表面膜的电位很可能会发生改变。本文首次报导：应用细胞电泳技术（ｃｅｌｌ ｅｌｅｃｔｒｏｐｈｏｒｅｓｉｓ）对细胞毒素类药物放线菌酮（ｃｙｃｌｏｈｅｘｉｍｉｄｅ）、放线菌素 Ｄ（ａｃｔｉｎｏｍｙｃｉｎ Ｄ）和秋水仙碱（ｃｏｌｃｈｉｃｉｎｅ）等诱导的植物凋亡细胞与正常细胞之间电泳迁移率（ＥＰＭ）的差异进行了比较,对引起的膜电位变化进行了定量分析。实验以玉米根尖分生组织为材料,制备原生质体,经过适当剂量的药物处理（Ｆｉｇ．１－Ｂ）,在尽量减少细胞膜被破坏的情况下（Ｆｉｇ．２）,观察到：三种细胞毒素类药物的作用有所不同,被诱导的植物凋亡细胞的膜表面Ｚｅｔａ电位绝对值比正常细胞的高（Ｆｉｇ．１－Ａ）。本研究提示细胞电泳可对凋亡细胞表面膜电位的变化进行定量分析,为细胞凋亡的检测在方法上提供了新思路。     

紫外辐射诱导烟草原生质体中DNA损伤的彗星电泳检测

以烟草原生质体为材料,采用彗星电泳检测用0.5W·m^-2紫外线以不同时间（0、5、10、30、60和120s）诱导的烟草原生质体中DNA的损伤。结果表明,在0～10s的时间内代表DNA损伤程度的尾矩、Olive尾矩等参数与紫外线照射时间具有良好的时间依赖关系。本文建立的烟草原生质体体系采用彗星电泳技术,可以快速而灵敏地检测紫外线对植物细胞的损伤程度。     

细胞凋亡原位检测的TUNEL法

细胞凋亡原位检测的ＴＵＮＥＬ法刘勇（江西省人民医院病理科,南昌３３０００６）细胞凋亡（ａｐｏｐｔｏｓｉｓ）,又称程序性细胞死亡（ｐｒｏｇｒａｍｍｅｄｃｅｌｄｅａｔｈ,ＰＣＤ）,是细胞的一种生理性死亡过程,有关细胞凋亡的研究近年来受到高度重视。末端转移...     

药物诱导的玉米根尖凋亡细胞表面电特性研究

细胞凋亡过程中细胞表面膜的电位很可能会发生改变。本文首次报导：应用细胞电泳技术（cell electrophoresis)对细胞毒素类药物放线菌酮（cycloheximide)、放线菌素D（actinomycin D）和秋水仙碱（colchicine)等诱导的植物凋亡的细胞与正常细胞之间电泳迁移率（EPM）的差异进行了比较,对引起的膜电位变化进行了定量分析。实验以玉米根尖分生组织为材料,制备原生质体,经过适当剂量的药物处理（Fig.1-B),在尽量减少细胞膜被破坏的情况下（Fig.2),观察到：三种细胞毒素类药物的作用有所不同。被诱导的植物凋亡细胞的膜表面Zeta电位绝对值比正常细胞的高（Fig.1-A)。本研究提示细胞电泳可对凋亡细胞表面膜电位的变化进行定量分析,为细胞凋亡的检测在方法上提供了新思路。     

羟自由基诱导烟草细胞凋亡

用适当浓度组合的硫酸亚铁和过氧化氢反应以产生羟自由基来处理烟草悬浮细胞,首次观察到了细胞中染色质凝缩、边缘化、细胞核解体等典型的细胞凋亡的形态学特征;在ＤＮＡ 琼脂糖凝胶电泳图谱上观察到因核ＤＮＡ 有规则地在核小体间被降解而产生的阶梯状条带;末端脱氧核糖核酸转移酶介导的３’ＯＨ 末端标记法（ｔｅｒｍｉｎａｌ ｄｅｏｘｙｎｕｃｌｅｏｔｉｄｙｌ ｔｒａｎｓｆｅｒａｓｅ （ＴｄＴ）ｍｅｄｉａｔｅｄ ｄＵＴＰ ｎｉｃｋｅｎｄｌａｂｅｌｉｎｇ,ＴＵＮＥＬ） 检测结果为阳性。这些实验表明,羟自由基确能诱导烟草细胞凋亡。     

爪哇伪枝藻胞外多糖诱导皮肤癌细胞(A431)凋亡的研究

为探讨爪哇伪枝藻胞外多糖(Extracellular polymeric substances of Scytonema javanicum, EPS)诱导人表皮癌A431细胞凋亡及其对凋亡相关基因caspase-3、bcl-2和bax表达的影响,本实验利用MTT法检测细胞生长抑制情况;HE染色法及透射电镜进行形态学观察;单细胞凝胶电泳法(SCGE/彗星电泳)分析DNA受损情况;免疫组织化学法检测细胞内caspase-3、bcl-2和bax表达水平。结果显示EPS能显著抑制A431细胞增殖,并呈时间和剂量依赖性,作用96h的半数抑制浓度IC50为4.25mg/mL,并出现细胞凋亡的形态学改变;彗星电泳结果与对照相比6mg/mL EPS作用48h能引起A431细胞DNA严重损伤;免疫组织化学检测发现6mg/mL EPS作用72h能显著上调A431细胞内凋亡相关基因caspase-3和bax的表达,而下调bcl-2的表达。     

Application of Comet Assay in Plant Protoplast Apoptosis Detection

The authors report the application of neutral comet assay in the detection of apoptosis in tobacco (Nicotiana tabacum L. ) pretoplasts. The results suggested a close inter-relationship between comet formation and nuclear compacting into densed masses at the nuclear periphery (a typical morphological symptom of apoptosis). Standard detection of hallmarks of apoptosis, including DNA laddering and TdT-mediated biotin-dUTP nick end-Lase Labeling (TUNEL), was also performed in order to conform the reliability of comet assay in the detection of apoptosis in plant protoplasts.     

Effect of ethrel on apoptosis in carrot protoplasts

In recent years, apoptosis has been reported to exist in plants during normal development and in response to stress. However, little is known about the relation of hormones to this form of programmed cell death. Here, we report examination of characteristics of apoptosis in carrot protoplasts induced by ethylene evolved from ethrel (2-chloroethylphosphonic acid). Nucleus condensation and DNA ladders were observed, and neutral comet assay, which detects DNA cleavage, also provided evidence that ethrel treatment resulted in nuclear DNA fragmentation. Strikingly, a close correlation between the incidence of DNA comets and the percentage of apoptotic protoplasts was shown in ethrel-treated carrot protoplasts. In conclusion, this study demonstrated that ethylene is an active inducer of apoptosis in carrot protoplasts, and that ethylene-induced plant cell death showed characteristics similar to those of apoptosis in animals.     

Aspects of programmed cell death during leaf senescence of mono- and dicotyledonous plants

Summary Leaf senescence is a highly regulated stage in the plant life cycle, leading to cell death, recently examined as a type of the programmed cell death (PCD). One of the basic features of PCD is the condensation of nuclear chromatin which is caused by endonucleolytic degradation of nuclear DNA (nDNA). In our investigations, we applied the technique of the single-cell electrophoresis system (“comet assay”) in order to determine the type of nDNA fragmentation during leaf senescence. The comet assay, a sensitive method revealing nonrandom internucleosomal damage that is specific for PCD, is especially useful for the detection of nDNA degradation in isolated viable cells. Simultaneously, we analyzed the mesophyll cell ultrastructure and the photosynthetic-pigment concentration in the leaves of two species,Ornithogalum virens andNicotiana tabacum, representing mono- and dicotyledonous plants which differ in the pattern of leaf differentiation. These investigations demonstrated that, in both species, the comet assay revealed nDNA degradation in yellow-leaf protoplasts containing chloroplasts that showed already changed ultrastructure (swelled or completely degraded thylakoids) and cell nuclei with a significant condensation of chromatin. There was no nDNA degradation in green-leaf protoplasts containing differentiated chloroplasts with numerous grana stacks and nuclei with dispersed chromatin. The analysis of intermediate developmental stage showed that the degradation of nDNA precedes condensation of nuclear chromatin. Thus the comet assay is a very useful and sensitive method for early detection of PCD. Moreover, results of our studies indicate that leaf senescence involves PCD.     

Comparison of comet assay, electron microscopy, and flow cytometry for detection of apoptosis.

Differentiating apoptosis from necrosis is a challenge in single cells and in parenchymal tissues. The techniques available, including in situ TUNEL (Terminal deoxyribonucleotide transferase-mediated dUTP-X Nick End-Labeling) staining, DNA ladder assay, and flow cytometry, suffer from low sensitivity or from a high false-positive rate. This study, using a Jurkat cell model, initially evaluated the specificity of the neutral comet assay and flow cytometry compared to the gold standard, electron microscopy, for detection of apoptosis and necrosis. Neutral comet assay distinguished apoptosis from necrosis in Jurkat cells, as evidenced by the increased comet score in apoptotic cells and the almost zero comet score in necrotic cells. These findings were consistent with those of electron microscopy and flow cytometry. Furthermore, using rats with burn or ischemia/reperfusion injury, well-established models of skeletal and cardiac muscle tissue apoptosis, respectively, we applied the comet assay to detect apoptosis in these muscles. Neutral comet assay was able to detect apoptotic changes in both models. In the muscle samples from rats with burn or ischemia-reperfusion injury, the comet score was higher than that of muscle samples from their respective controls. These studies confirm the consistency of the comet assay for detection of apoptosis in single cells and provide evidence for its applicability as an additional method to detect apoptosis in parenchymal cells.     

Comet assay and DNA flow cytometry analysis of staurosporine-induced apoptosis.

BACKGROUND: The ability of the comet assay to quantify DNA strand breaks and alkali labile sites has been widely demonstrated. In this study, this assay was tested for its ability to identify DNA fragmentation occurring during apoptosis in comparison with standard DNA flow cytometry analysis. METHODS: Staurosporine-induced apoptosis in CHO cells is an adequate model to study a rapid time- and dose-dependent appearance of this process. RESULTS: Nuclear staining with DAPI confirmed the induction of apoptosis with a typical chromatin condensation and fragmentation. Analysis of propidium-iodide- (PI) stained DNA by flow cytometry showed the presence of a pre-G1 peak, characteristic of apoptotic cells, 6 h after drug treatment. The detection of highly damaged cells (HDC) by the comet assay after 3 h treatment occurred earlier than the detection of apoptotic cells by flow cytometry. However, HDC were missed when the DNA fragmentation was too high, preventing accurate quantification of late apoptotic cells. CONCLUSIONS: The comet assay is more sensitive than standard DNA flow cytometry to detect early DNA fragmentation events occurring during apoptosis. However, the comet assay modified by omitting electrophoresis was necessary to quantify apoptotic fraction at later stages.     

Induced cell death of preimplantation mouse embryos cultured in vitro evaluated by comet assay

The occurrence of apoptosis in mouse preimplantation embryos was analyzed using DNA staining (Hoechst 33342, PI) for the visualization of nuclear changes and by the comet assay, a single-cell gel electrophoresis assay, modified for the analysis of blastocysts. Mouse preimplantation embryos isolated 56 h after superovulation were cultured in vitro for 64 h. Apoptosis was induced by treatment with camptothecin and actinomycin D during the first 15 h of culture. After culture in vitro, a number of embryos were stained and analyzed using morphological criteria. The remaining embryos were examined using the comet assay for the detection of DNA fragmentation. The proportion of damaged embryos in experimental groups, in comparison to controls, was dependent on the dose of apoptosis inductor. At high doses (camptothecin, microg/ml and actinomycin D, 0.05 microg/ml) over 90% (chi-square test, P<0.001) of embryos had apoptotic comets, at medium doses (camptothecin, 0.01 microg/ml and actinomycin D, 0.005 microg/ml) comets appeared only in 30-70% of embryos (camptothecin, P<0.01 and actinomycin D, P<0.001). At low doses (camptothecin, 0.001 microg/ml and actinomycin D, 0.0005 microg/ml) the increase in damaged embryos was not statistically significant. Hoechst/PI staining showed a higher percentage of damaged blastomeres at high doses. Morphological changes correlated with the outcome of the comet assay. Our results show that comet assay is an appropriate method for studying apoptosis in preimplantation embryos, and it appears to be more sensitive than the classically used morphological analyses.     

A first step in visual identification of different cell populations by a modified alkaline comet assay

Using a particular model of apoptosis, we here demonstrate the ability of the comet assay to differentiate between different cell populations. In our study, the natural killer Kurloff cells, used as effector cells, recognize and bind to the tumoral L2C target cells. Formation of such conjugates leads to the death of the target cells by apoptosis, as previously described by different conventional techniques. With the alkaline comet assay, a conjugate could directly be visualized as an association of an undamaged cell joined to a highly damaged cell. The modified comet assay used in this study comprises specific labelling of Kurloff cells with immunomagnetic beads, which are visible as grey-dull spheres against the bright-red staining of nuclear origin on the comet preparation. The use of such labelled effector cells suggest the potential of the comet assay to visually identify different cell populations in an unique test.