DNA measurements of cervical epithelial cells in combination with scanning electron microscopy

A method is described in which the surface morphology of benign and malignant cervical cells is investigated with a combined light microscope-scanning electron microscope, after the measurement of the DNA content of each individual cell in the same instrument. The suspect cells can thus be identified by an increased aneuploid DNA content (greater than 5C) and not primarily by morphology. The DNA content was measured, after a quantitative acriflavine-Feulgen staining, by using a microphotometer attached to the combined microscope. It was found that the suspect cells show a different surface morphology compared to normal cells from a benign specimen.     

Cell surface characteristics and DNA content of macrophages in murine bone marrow cultures

Summary An instrument combining scanning electron microscopy (SEM) and light microscopy (LM) was used to study the cell surface characteristics and DNA content of macrophages in murine bone marrow cultures. After a quantitative Feulgen DNA staining, the DNA content of the individual macrophages was measured and their cell surface morphology was studied immediately thereafter with the SEM part of the instrument. The cells were divided into six groups according to the number of microvilli and/or microridges present on their surface. A proportion of macrophages showed a DNA content more than occurs in diploid cells, which could indicate a future division. No special surface morphology could be detected in this cell type.     

Cell surface characteristics and DNA content of macrophages in murine bone marrow cultures. A study using simultaneous scanning electron microscopy and fluorescence microscopy

An instrument combining scanning electron microscopy (SEM) and light microscopy (LM) was used to study the cell surface characteristics and DNA content of macrophages in murine bone marrow cultures. After a quantitative Feulgen DNA staining, the DNA content of the individual macrophages was measured and their cell surface morphology was studied immediately thereafter with the SEM part of the instrument. The cells were divided into six groups according to the number of microvilli and/or microridges present on their surface. A proportion of macrophages showed a DNA content more than occurs in diploid cells, which could indicate a future division. No special surface morphology could be detected in this cell type.     

Flow cytometric determination of DNA content in malignant and benign bone tumours

The nuclear DNA content of 38 malignant and 25 benign bone tumours was measured by flow cytometry. The specimens were taken either from biopsies or from surgical specimens. Seventeen of 26 primary malignant bone tumours were aneuploid, 15 had a single aneuploid DNA content, and 2 had a biclonal abnormality. Thirteen of 15 osteosarcomas were aneuploid, but only 2 of 6 chondrosarcomas showed an aneuploid DNA content. Six of 12 metastatic malignant bone tumours were also aneuploid. All 25 benign tumours had a diploid DNA content. Cell cycle analysis showed that the proportion of cells in S- and G2M-phases was higher in the malignant compared to benign tumours, indicating a higher proliferative activity. The increase was statistically significant (p less than 0.05) both in diploid and in aneuploid tumours. Among five tumours studied after chemotherapy, four displayed a marked hyperdiploid abnormality. Aneuploidy and high proliferative activity both were highly associated with malignant bone tumours, suggesting that DNA flow cytometry may be an adjunct in the assessment of malignancy of bone tumours.     

De novo pyrimidine nucleotide biosynthesis in synchronized rat hepatoma (HTC) cells and mouse embryo fibroblast (3T3) cells.

We studied the effect of cellular concentration on the intensity of fluorescence of AO-stained cells according to Rigler. The cell concentration in the preparations of human leukocytes was changed after fixation, i.e. any possibility of alteration of the functional state of chromatin was precluded. For this purpose two methods were used: (1) the cells were washed from the surface of the fixed preparation by high pressure stream of fixative; (2) the greater part of the cells attached to the slide was removed with a razor blade. A comparative study of cell morphology in intact preparations and in preparations with reduced cell content was done by electron microscopy. The DNA content of the lymphocytes remaining on the slide after treatment with the fixative and of lymphocytes of intact preparations was determined by Feulgen cytophotometry.It was found that the intensity of fluorescence of AO-stained cells was dependent upon the cell concentration on the surface of the coverslip. Thus it was not caused by a change in the functional state of the cells. This dependence could not be accounted for, either by the DNA deficit or by morphological alterations in the cells remaining on the slide after partial removal by these methods. The experiments showed that the process of dye diffusion from the cells was influenced by the concentration of cells on the slide. The possibilities of avoiding these errors are discussed.     

Fusion of mammalian oocytes: SEM observations of surface changes

Mouse oocytes at the germinal vesicle (GV) stage were fused with maturing oocytes in which GVs were no longer visible. The fused cells were fixed at different time-intervals after the initiation of fusion and prepared for scanning electron microscope (SEM) observation. Concomitantly, some fused cells were prepared for light microscope evaluation. Our SEM observations showed no significant differences in surface morphology between immature and maturing oocytes. However, immediately after fusion was initiated, dramatic changes occurred on the surface of the maturing oocytes. The microvilli were shortened or disappeared locally and the plasma membrane was deeply ruffled. One hour after fusion, when the giant cells were nearly spherical, the microvilli reappeared and the ruffling gradually disappeared. In some areas, the microvilli were extremely long. Three hours after fusion, the fused cells were perfectly round and their surfaces were generally covered with microvilli of equal length. No further ruffling was observed. It is suggested that cytoplasmic mechanisms regulate the surface morphology of the oocytes during fusion.     

Procedure for isolating micronuclei from rat kangaroo cultured cells containing individualized chromosomes

Micronuclei are small interphase nuclei containing part of the genome; the DNA content of the smallest micronuclei is equivalent to one chromosome. For analysis by biochemical method and by cytofluorometry of interphase micronuclei containing a single chromosome, several isolation and purification procedures were tested and checked by fluorescent microscopy using the DNA dye Hoechst 33 342 and electron microscopy. Micronucleation of rat kangaroo epithelial cells was induced by colchicine treatment for three days. Micronuclei were isolated in a low ionic strength buffer containing collagenase, with concomitant mechanical shocks. Eighty % of the micronuclei were released after 3 to 7 min, with minimum nuclear breakage. Subsequent filtration through several polycarbonate filters 12, 8 and 5 micron in diameter enabled purification of the smallest micronuclei without aggregates or debris. Micronuclear morphology was well preserved, as shown by electron microscope observations. Therefore, we established the optimal conditions allowing gentle mass isolation of individual micronuclei of cultured PtK1 cells, compatible with flow cytometry analysis.     

二氧化氯对球形棕囊藻叶绿素a、蛋白质、DNA含量的影响

分析了二氧化氯(1.0、1.5、2.0、2.5mgL-1,作用96h;2.5、6.0、8.0、16.0mgL-1,作用60min)对球形棕囊藻叶绿素a、蛋白质含量、氨基酸组成、核酸含量的影响,用透视电镜对二氧化氯(0.5mgL-1,0.8mgL-1)作用24h后藻细胞形态的变化进行了观察,以探讨二氧化氯去除赤潮藻的机理。结果表明,二氧化氯对球形棕囊藻叶绿素a、蛋白质、DNA的含量均有影响。实验各组(1.0-2.5mgL-1,2.5-16.0mgL-1)球形棕囊藻的叶绿素a、蛋白质、DNA的含量均显著低于对照。二氧化氯浓度超过2mgL-1时,球形棕囊藻的叶绿素a、蛋白质、DNA的含量持续降低,氨基酸相对含量发生明显变化;半胱氨酸、酪氨酸和赖氨酸等的相对含量明显降低,而组氨酸、缬氨酸和苯丙氨酸则明显增加。当二氧化氯(2.5-16.0mgL-1)作用3min后,DNA漏出率在13%-18%之间;电镜观察发现,二氧化氯可使细胞膜破损,引起内容物外泄。这些结果显示,二氧化氯能以单分子形式进入细胞,引起叶绿素、蛋白质结构的变化,并破坏藻细胞膜系统,最终导致藻细胞死亡。     

THE HISTOCHEMISTRY AND ULTRASTRUCTURE OF JACK PINE MICROSPORANGIA DURING THE WINTER

The development of jack pine (Pinus banksiana Lamb.) microsporangia from October to April was investigated with a microdensitometer and a transmission electron microscope. DNA, RNA, and protein content of sporogenous cells was measured at monthly intervals. DNA was unreplicated (2C) until March when DNA synthesis was first noted, coinciding with a loss of heterochromatin. Protein content doubled in April. RNA staining increased in December and then decreased. Numerous whorls and stacks of rough endoplasmic reticulum and ribonucleoprotein-like granules appeared in December and may be related to the RNA increase. A fibrillar, light-staining region was found in the cytoplasm of the sporogenous cells from November to March. It was hydrolyzed in the presence of protease and may be a winter morphology of microfilament bundles or dictyosomes. Lipid bodies and vacuoles were abundant in the tapetum and sporangial wall cells during the winter. Observations substantiate reports that winter is not a time for cessation of development.     

Distinction of apoptotic and necrotic cell death by in situ labelling of fragmented DNA

The occurrence and spatial distribution of intracellular DNA fragmentation was investigated by in situ 3 end labelling of DNA breaks in K562 cells treated in such a way to cause either apoptotic or necrotic cell death. The localisation of DNA breaks was examined by confocal laser microscopy and compared with the electron-microscopic appearance of the cells. In addition, the number of cells with fragmented DNA was counted and compared with the number of dead cells, as determined by the nigrosin dye exclusion test. Apoptosis was induced by cultivation of the cells in the presence of actinomycin D. Cells undergoing apoptosis were characterised by massive intracellular DNA fragmentation that was highly ordered into successive steps. Cells in early stages of the apoptotic process had DNA breaks diffusely distributed in the entire nucleus, except the nucleolus, with crescent-like accumulations beyond the nuclear membrane. In the more advanced stages, the nucleus was transformed into many round bodies with intense labelling. Intracellular accumulations of fragmented DNA corresponded exactly to electron-dense chromatin seen in the electron microscope, whereas diffuse DNA breaks had no morphological correlate at the ultrastructural level. In necrosis induced by ionomycin, NaN₃, or rapid freezing combined with thawing, no DNA fragmentation occurred at the onset of cell death, but appeared 24 h later. This fragmentation was not characterised by a unique morphology, but represented the breakdown of the chromatin in the configuration remaining after cell death. Therefore, apoptosis is characterised by DNA fragmentation that proceeds in a regular orderly sequence at the beginning of cell death, and can be detected by in situ 3end labelling of DNA breaks.     

超声波介导质粒pET28a转化枯草芽胞杆菌的研究

揭示超声波介导下质粒DNA转化枯草芽胞杆菌发生的生物学机制,以便于枯草芽胞杆菌基因工程菌株的工业化应用。建立超声波介导质粒pET28a转化枯草芽胞杆菌的一种方法,采用扫描电镜结合理化分析检测技术研究超声波处理前后细胞的变化。结果显示,一定条件的超声(40~100 W)处理后的质粒DNA可以转化枯草芽胞杆菌,处理后的细胞在电镜下表面凹凸不平,出现褶皱现象;而且胞内蛋白质、磷脂及碱性磷酸酶(AP)大量释放至胞外。结果表明,超声波介导的DNA转化是细胞生理响应与超声波共同作用的结果。     

神经生长因子对PC12细胞脂多糖损伤的保护作用及其机制

目的：细胞水平研究神经生长因子（NGF）对大鼠嗜铬细胞瘤细胞株（PC12细胞）脂多糖（LPS）损伤后的保护作用以及核转录因子（NF-κB）的活性影响,探讨药物作用机制。方法：PC12细胞常规培养后,建立LPS损伤模型,随后MTT观察不同浓度的LPS对PC12细胞损伤及NGF对LPS损伤的保护作用,同时用倒置显微镜和荧光显微镜下观察细胞状态,最后RT-PCR检测NF-κB的含量。结果：①PC12细胞LPS损伤有浓度梯度,随着LPS浓度的增加,PC12细胞的存活率不断下降;LPS损伤的同时加入不同浓度NGF,LPS损伤均有明显的改善。②显微镜观察显示PC12细胞形态学上的改变,表明NGF对LPS损伤有保护作用。③RT-PCR结果显示,LPS损伤细胞的NF-κB的相对表达量明显高于正常对照细胞,而药物治疗组的NF-κB表达量则接近于正常细胞。结论：目前,神经生长因子在脑内炎症后的细胞修复作用报道甚少,而本实验研究神经生长因子对PC12细胞LPS损伤起到保护作用,尤其是损伤后再修复作用,且其作用机制可能与NF-κB信号通路的调控有关。     

休克淋巴液对大鼠肺微血管内皮细胞的损伤作用

无菌条件下复制大鼠重症失血性休克模型,引流肠系膜淋巴液或收集门静脉血,同时,引流正常淋巴液、正常门静脉血。以不同处理因素与原代培养的第三代肺微血管内皮细胞(PMVEC)共同孵育,通过光镜、透射电镜、扫描电镜观察细胞形态及超微结构,MTT法检测不同终浓度的休克淋巴液及正常淋巴液对PMVEC增殖的影响;流式细胞仪检测PMVEC周期变化;同时进行细胞核DNA电泳分析。结果表明,休克淋巴液对PMVEC具有损伤作用,表现为细胞收缩、核固缩等,扫描电镜可观察到凋亡小体;随着休克淋巴液终浓度增加,PMVEC的增殖活力逐渐降低,显著低于正常淋巴液组;4%终浓度的休克淋巴液作用PMVEC 4h后,G0-G1期细胞比值增大,S G2-M期细胞比值下降,其他处理因素无明显变化,同时细胞核DNA电泳形成典型的阶梯状电泳图谱(DNA ladder)。结果提示,休克淋巴液可导致PMVEC形态学及超微结构损伤,同时抑制细胞增殖、影响细胞周期、诱导细胞凋亡。     

A molecular delivery system by using AFM and nanoneedle

We developed a new low invasive cell manipulation and gene or molecule transfer system in a single living cell by using an atomic force microscope (AFM) and ultra thin needle, a nanoneedle. DNA was immobilized on the surface of the nanoneedle by covalent bonding and avidin-biotin affinity binding. Immobilization of DNA on the nanoneedle was confirmed by measuring the unbinding force between avidin and biotin. The DNA-immobilized nanoneedle was successfully inserted into HEK293 cells. Though TO-PRO-3 iodide staining experiments using confocal microscopy, we observed the immobilized DNA on the surface of the nanoneedle, which was retained after 10 times insertions to and evacuations from a living cell.     

Proliferative characteristics and ploidy of human brain tumors by DNA flow cytometry

We studied nuclear DNA distribution by flow cytometry in 59 human brain tumors. Samples were frozen at -20 degrees C immediately after surgery and unicellular suspensions were obtained with a mechanical dissociation technique. Nuclear DNA was stained with propidium iodide. Normal human brain tissue was used as a diploid reference standard. In 86.3% of benign tumors an unimodal DNA distribution with a DNA index usually within the diploid range was found. Among malignant tumors, 64% had un unimodal DNA distribution with diploid or near-diploid modal DNA content. The remaining 36% showed an additional cell peak with a DNA index ranging from 1.15 to 1.92. The percentage of S-phase cells was higher in malignant (median = 3.8) than in benign tumors (median = 1.9) (p less than .001), without correlation to histological tumor subtype.     

Restricted amino acid nutrition induces attachment to glass and spreading of Ehrlich ascites tumour cells

Ehrlich ascites tumour (EAT) cells were cultured in vitro in Eagle's MEM and Medium 199 with a lowered amino-acid content. Under these conditions EAT cells lose their rounded shape typical of highly malignant cancer cells, and begin to spread on the substratum. The changes in EAT cell morphology are preceded by a decrease in the rate of protein synthesis. These changes were maintained for three days after returning the cells to Eagle's MEM with a normal amino-acid content, but the return to control media did not cause reasumption of growth in the once spread cells. The increase in glucose content (up to five-fold) or the presence of inhibitors of DNA synthesis did not prevent the attachment and flattening of EAT cells in media with a lowered amino acid content. Several possible mechanisms of the influence of restricted amino-acid availability on the changes in EAT cell surface properties are pointed out and the need for study of cancer cell responses to restricted nutrition is discussed.     

Measurement of DNA content in single cells morphologically identified on smears

A method was developed for measuring the nuclear DNA content in single cells previously identified on a bone marrow smear stained by the Wright-Giemsa method. The smear was first photographed and the location of individual cells, identified by morphology, was recorded on a cell map. The smear was then bleached with 50% acid ethanol and absolute methanol, and re-stained by the Feulgen method in 0.05% pararosaniline Schiff's reagent (pH 2.3) at 7 degrees C for 10 min. Nuclear red fluorescence was observed and the intensity of this fluorescence was proportional to the amount of DNA after prior irradiation of smears with green light for 9 hr. The method is useful for measuring cell DNA content in heterogeneous cell populations when morphological cell identification is required.     

DNA content by in situ fluorescence imaging and S-phase detection, with chromatin structure preserved

OBJECTIVE: To test the feasibility of in situ DNA quantitation of adherent cells' nuclei by fluorescence imaging, preserving chromatin structure and to follow-up S phase, in relation to DNA content, in order to assess the precision of DNA measurements. STUDY DESIGN: Double labeling experiments involved total DNA staining with Hoechst 33342 and BrdU immunostaining (after either Br photolysis and DNA strand break labeling by terminal transferase or acid denaturation) to detect replicating DNA. An epifluorescence microscope was used, images captured with a CCD camera and quantitative total DNA measurements done in 12 bits with IPLab software. BrdU results were related to DNA content on an individual cell basis. Cell cycle analyses were run with Imastat software (developed in the laboratory) on Hoechst-stained cells and on double labeled cells. RESULTS: In cells progressing through the cycle, as assessed by BrdU, a corresponding increase in DNA content was measured. Early S differed from G1 (P < .05). Imastat analyses gave a CV for GI peak of 6-7%. CONCLUSION: Quantitative fluorescence imaging allows a sensitive determination of DNA content for adherent-cell nuclei in situ. Topologic analyses of nuclear components will be possible in relation to DNA content.     

DNA flow cytometry of breast carcinoma after acetic-acid fixation

Aqueous acetic acid was used to fix and store specimens of tissue prior to dissociation into nuclear suspensions for flow cytometric quantitation of DNA. The optimum concentration was 20 volumes of glacial acetic acid in 80 volumes of distilled water. Both neoplastic and benign nuclei were easily released from the fixed tissue blocks by slicing and shaking. Residual undissociated tissue was suitable for microscopic examination to confirm its identity. The nuclei fluoresced brightly after staining with propidium iodide, and yielded histograms similar to those from unfixed samples. Acetic-acid fixation resulted in slightly broader G1 and G0 peaks in the DNA histograms in comparison to unfixed cells, but fluorescent debris was less and correlation between the flow cytometric S-phase fraction (SPF) and in vitro thymidine labelling index (TLI) was better than with unfixed cells. Twenty-one of thirty-nine acetic-acid-fixed breast carcinomas had DNA indices in excess of 1.0 (increased nuclear DNA content in comparison to benign cells), and eighteen had DNA indices of 1.0 (normal or near-normal). The SPF was usually in excess of the TLI, but the two were significantly correlated (r = 0.72, P less than 0.0001). However, a significant correlation of SPF with TLI held only for the group with DNA index greater than 1.0. DNA indices greater than 1.0 were associated with high SPF and TLI, and high SPF and TLI each associated with low content of estrogen receptor.