Association between Tumorigenic Potential and the Fate of Cancer Cells in a Syngeneic Melanoma Model

The self-renewal potential of a cancer cell can be estimated by using particular assays, which include xenotransplantation in immunocompromised animals or culturing in non-adherent serum-free stem-cells media (SCM). However, whether cells with self-renewal potential actually contribute to disease is unknown. Here we investigated the tumorigenic potential and fate of cancer cells in an in-vivo melanoma model. We examined cell lines which were derived from the same parental line: a non-metastatic cell line (K1735/16), a metastatic cell line (K1735/M4) and a cell line which was selected in non-adherent conditions (K1735/16S). All cell lines exhibited similar proliferation kinetics when grown on culture plates. K1735/16 cells grown in soft agar or in suspension non-adherent conditions failed to form colonies or spheroids, whereas the other cell lines showed prominent colonogenicity and spheroid formation capacity. By using sphere limiting dilution analysis (SLDA) in serum-free media, K1735/16S and K1735/M4 cells grown in suspension were capable of forming spheroids even in low frequencies of concentrations, as opposed to K1735/16 cells. The tumorigenic potential of the cell lines was determined in SCID mice using intra footpad injections. Palpable tumors were evident in all mice. In agreement with the in-vitro studies, the K1735/M4 cell line exhibited the highest growth kinetics, followed by the K1735/16S cell line, whereas the K1735/16 cell line had the lowest tumor growth potential (P<0.001). In contrast, when we repeated the experiments in syngeneic C3H/HeN mice, the K1735/16 cell line produced macroscopic tumors 30–100 days after injection, whereas K1735/M4 and K1735/16S derived tumors regressed spontaneously in 90–100% of mice. TUNEL analysis revealed significantly higher number of apoptotic cells in K1735/16S and K1735/M4 cell line-derived tumors compared to K1735/16 tumors (P<0.001). The models we have examined here raised the possibility, that cells with high-tumorigenic activity may be more immunogenic and hence are more susceptible to immune-regulation.     

The influence of ethanol on cell membrane fluidity, migration, and invasion of murine melanoma cells

The short-term effects of ethanol (85.4, 170.8, and 256.2 mM) on cellular viability, proliferation, migration, and invasion were investigated on murine melanoma cells. Experiments with the fluorescent probe 1,6-diphenyl-1,3,5-hexatriene indicated that the two highest concentrations of ethanol induced low microviscosity (high lipid fluidity). Cellular viability and proliferation, as determined by the incorporation of [3H]IdUR, were unaffected by all three concentrations of ethanol. A membrane migration assay and a collagen type IV invasion assay evaluated cellular migration and invasion, respectively. For B16F10 and K1735 cells, the migration rate was significantly increased by 170.8 and 256.2 mM concentrations of ethanol. Although the invasion of B16F10 cells was not affected, invasion of K1735 cells was inhibited by 170.8 and 256.2 mM ethanol. The effect of ethanol on the cytoskeleton was monitored by fluorescent staining of F-actin. In contrast to untreated cells, F-actin staining of 256.2 mM ethanol-treated cells showed spike-like projections from the cell surface. Our findings suggest that ethanol can influence cell migration and invasion in vitro, as well as F-actin organization.     

Proportion of antigenic variants induced by in vitro UV irradiation differs in clones derived from a single tumor

The purpose of this study was to examine the capacity of different clones derived from the same tumor to generate highly antigenic cells after in vitro exposure to UV radiation. Cells from the metastatic murine melanoma K1735 and clones of K1735 differing in metastatic potential were exposed to UV radiation in vitro, cloned, and tested for antigenic properties in vivo. Approximately half of the clones isolated after UV irradiation of parental K1735 melanoma cells were highly antigenic (five of nine). Similar treatment of cells of a nonmetastatic clone of K1735 generated clones that were all antigenic (nine of nine). In contrast, only one of nine clones derived from UV-irradiated cells of a highly metastatic clone of K1735 were antigenic. Clones derived from unirradiated cultures were not antigenic variants. The increased antigenicity of cells derived from UV-irradiated cultures did not correlate with an increase in expression of cell surface class I major histocompatibility complex antigens. These results demonstrate that the frequency of antigenic variant production after UV irradiation is an intrinsic property of the particular cell line used, and that even cloned cell lines derived from a single tumor differ in their ability to generate antigenic variants after UV irradiation. In addition, they indicate that the increased antigenicity is not necessarily due to a UV-induced increase in expression of cell surface class I histocompatibility antigens.     

Parasitism of monolayer cultures of dog tissue by Histoplasma capsulatum,I preliminary investigations

Summary Monolayer tissue cultures of canine kidney are demonstrated to by susceptible to invasion by yeast-phaseHistoplasma capsulatum. Primary and secondary tissue cultures of canine kidney show different levels of invasion by the pathogen at 24 hours after inoculation; these differences are interpreted as being related to the number of dividing host cells. By 72 hours after inoculation, similar numbers of yeast cells are demonstrable within the host cells of primary and secondary cultures. Essentially identical results were obtained when canine heart tissue cultures were inoculated with y-phaseH. capsulatum.Paper No.713, Department of Botany and Plant Pathology, The Ohio State University, 1735 Neil Avenue, Columbus 10, Ohio; correspondence should be directed to the junior author at the above address.     

北京东灵山地区辽东栎林种群空间分布分形分析

通过植物个体的坐标点与模拟冠幅的分形维数的分析,对辽东栎林内不同种群沿海拔梯度变化的空间分布格局和种群动态进行了比较和讨论。结果表明:模拟冠幅分形分析方法更适于分析具有大小不等、复杂多样的冠幅的植物个体空间分布格局。随着海拔的升高,不同种群的空间占据能力也随之变化。辽东栎种群的空间分布占绝对优势地位,分形维数可达1.9811;五角枫种群则逐步下降,分形维数最低为0.1170。低海拔山坡六道木种群空间占据能力较强,高海拔山坡照山白种群有较大的空间占据能力。在一定的环境条件下,不同的种群可能具有相近的空间占据能力,但对乔木层与灌木层来说,相同的分形维数的内涵是不同的。冠幅的分形维数作为表征植物种群空间占据能力的工具,是种群动态分析和种群分布格局研究的的重要指标之一。     

Non-small-cell lung carcinoma cells invade human bronchial mucosa In vitro

Summary To study invasion of lung cancer in vitro a novel three-dimensional coculture assay consisting of living human tissues has been developed. Multicellular spheroids initiated from a new large-cell lung carcinoma cell line (GaL23), found to be invasive in immunodeficient mice, were confronted with precultured bronchial fragments derived from mucosal biopsies obtained during routine fiberoptic bronchoscopy. The bronchial fragments consist of a stromal core with scattered fibroblasts covered by a continuous surface epithelium resting on a basal lamina. During the first 2 wk of confrontation, a gradual retraction of the bronchial epithelium with subsequent adhesion of the tumor cells to the underlying basal lamina occurred. The following week, a limited invasion of tumor cells into the bronchial stroma was seen. To facilitate the entrance of tumor cells through the mucosal surface, the surface epithelium was removed prior to coculture by ethylenediaminetetraacetic acid (EDTA) buffer treatment. Upon confrontation, GaL23 cells then rapidly attached to and migrated on the exposed basal lamina and an increasing number of tumor cells was seen in the stroma during the first week of culture. This model offers opportunities for studying mechanisms of lung cancer adhesion, migration, and invasion using human bronchial mucosa as the natural target tissue.     

The nature of host tissue destruction in tumor invasion. An experimental investigation on carcinoma and sarcoma xenotransplants

The nature of host tissue destruction in tumor invasion was investigated in experimentally induced carcinomas and sarcomas, xenografted into skeletal muscle. By means of light and electron microscopy it was shown that in both carcinomas and sarcomas the confrontation of host tissue with the invading tumor cells does not result in immediate destruction of host tissue but in a transitory state of coexistence which gradually proceeds to progressive host tissue atrophy. This process of progressive atrophy, which finally results in the total disappearance of the invaded host tissue, is considered to be caused mainly by the increasing pressure and competitive withdrawal of oxygen and nutrients by the invading and proliferating tumor cells. Morphological changes suggesting an active enzymatic breakdown of host tissue cells by tumor cells were not observed during any stage of tumor invasion.     

Analysis of fractal dimension of O2A glial cells differentiating in vitro

Fractal dimension is a quantitative measure of morphological complexity. Glial cells of the oligodendrocyte-type 2 astrocyte (O2A) lineage exhibit increasing morphological complexity as they differentiate in vitro. Enriched populations of O2A progenitor cells isolated from neonatal rat cerebral hemispheres or optic nerves were allowed to differentiate in vitro, and their fractal dimensions were measured over time. The fractal dimensions of the maturing cells correlated with perceived complexity; cells with elaborate process branching had larger fractal dimensions than cells with a simpler morphology. An analysis of changes in fractal dimension revealed distinct rates of growth for both oligodendrocytes and type 2 astrocytes. The fractal dimension remained constant over a 10-fold range in optical magnification, demonstrating that cultured O2A glial cells exhibit self-similarity, a defining characteristic of fractal objects. These results illustrate that fractal dimension analysis of maturing cell populations is a useful method for quantitatively describing the process of cell differentiation.     

Fractal geometric analysis of lung cancer angiogenic patterns

For medical images, the fractal dimension D may be used as an index of irregularity. The angiogenesis patterns of lung cancer were analysed by means of the perimeter-area and box counting algorithms. The fractal nature of all images in the sense of the perimeter-area method and of 68% images in the sense of the box-counting method suggest the possibility to use the fractal dimension as a new non-morphometric parameter evaluating angiogenic processes in neoplasms.     

细菌感染与Gasdermin家族介导的宿主细胞程序性死亡的研究进展

侵入宿主后,细菌生长、繁殖并与宿主相互作用,引发机体不同程度的病理变化。为抑制细菌致病过程,宿主免疫系统产生抗感染免疫应答,感染的发生和发展取决于细菌对机体的致病性与机体抗细菌免疫的相互抗争。在细菌所致感染性疾病的发生、发展过程中,细菌与宿主细胞的拮抗往往涉及程序性细胞死亡(programmed cell death, PCD)这一过程。新近发现Gasdermin家族成员Gasdermin D和Gasdermin E参与PCD过程,并在其中发挥重要作用,跟踪其研究进展将有助于应对细菌感染造成的威胁。     

Fractal dimension in aspiration cytology smears of breast and cervical lesions

OBJECTIVE: To standardize the automated measurement of fractal dimension on cytologic smears and compare the fractal dimension of benign and malignant breast cells and cervical lesions on cytologic material to evaluate its role in the discrimination of benign from malignant cells. STUDY DESIGN: We randomly selected fine needle aspiration cytology smears of 42 cases of infiltrating duct carcinoma and 38 cases of fibroadenoma of the breast. Similarly, 16 cervical carcinoma and 20 normal cervical smears were selected for study. Ten cells were selected randomly from each case. Box counting of fractal dimension of malignant and benign cells was achieved with an image cytometer (Leica, Cambridge, England) using Quantimet 600 software (Leica). Then a well-spaced grid with multiple small boxes of a particular pixel length was superimposed on the cell. The dimension of the box was selected as 4, 8 and 16 pixels. With the help of a logical "AND" operation, we counted the number of boxes touching the peripheral margin of the cell nuclei. For each cell, the log-log graph of 1 per box size was plotted against the number of boxes touching the peripheral rim of the cell. The slope of each graph was identified using the least-squares method of regression analysis. RESULTS: The mean fractal dimension of malignant cells was 0.8536 +/- 0.1120 as compared to 0.8403 +/- 0.1115 in benign cell groups. The Mann-Whitney U test showed a significant difference in fractal dimension in these 2 groups (P = .05). The mean fractal dimension of malignant cells from the cervix was 0.8656 +/- 0.1499 as compared to 0.8315 +/- 0.1312 in benign cells. The Mann-Whitney U test showed a significant difference in fractal dimension in these 2 groups (P < .02). CONCLUSION: Fractal dimension may be a helpful adjunctive technique to discriminate between benign and malignant cells.     

Fractal dimension of antibody‐PEG precipitate: Light microscopy for the reconstruction of 3D precipitate structures

Protein and in particular antibody precipitation by PEG is a cost‐effective alternative for the first capture step. The 3D structure of precipitates has a large impact on the process parameters for the recovery and dissolution, but current technologies for determination of precipitate structures are either very time consuming (cryo‐TEM) or only generate an average fractal dimension (light scattering). We developed a light microscopy based reconstruction of 3D structures of individual particles with a resolution of 0.1–0.2 µm and used this method to characterize particle populations generated by batch as well as continuous precipitation in different shear stress environments. The resulting precipitate structures show a broad distribution in terms of fractal dimension. While the average fractal dimension is significantly different for batch and continuous precipitation, the distribution is broad and samples overlap significantly. The precipitate flocs were monofractal from micro‐ to nanoscale showing a random but consistent nature of precipitate formation. We showed that the fractal dimension and 3D reconstruction is a valuable tool for characterization of protein precipitate processes. The current switch from batch to continuous manufacturing has to take the 3D structure and population of different protein precipitates into account in their design, engineering, and scale up.     

Induction of antitumor immunity after cure of pulmonary metastases, using staphylococcal enterotoxin B and bispecific antibody

The combination of staphylococcal enterotoxin B (SEB) and anti-p97 x anti-CD3 bispecific antibody (bsAb) cures 60%-80% of mice with established pulmonary metastases of the syngeneic p97+ murine melanoma, CL62. We investigated the ability of cured mice to generate protective antitumor immunity. In tumor rechallenge experiments, CL62-cured mice developed protective immunity against rechallenge with CL62. The majority of mice also rejected the p97-negative parental cell line, K1735, indicating an immune response to tumor antigens common to both cell lines that were not bsAb-targeted. A significant humoral response developed against p97 antigen, but not against other antigens common to both CL62 and K1735. That the majority of cured mice nevertheless rejected K1735 suggests that tumor immunity is not antibody-dependent. Evidence of cellular immunity was obtained from the results of delayed-type hypersensitivity, proliferation and cytotoxicity assays, which revealed the presence of tumor-specific memory in bsAb-treated, CL62-cured mice. CD8+ T cells from cured, but not control mice were able to lyse tumor; however, memory CD4 cells had no cytolytic function. In vivo, however, both CD4 and CD8 T cells were required for effective protective immunity. These studies demonstrate that treatment with SEB and bsAb not only confers passive immune effects of tumor eradication, but also actively promotes the generation of a host antitumor immune response.     

Trypanosoma cruzi: phosphatidylinositol 3-kinase and protein kinase B activation is associated with parasite invasion

Multiple signal transduction events are triggered in the host cell during invasion by the protozoan parasite Trypanosoma cruzi. Here, we report the regulation of host cell phosphatydilinositol 3-kinase (PI3K) and protein kinase B (PKB/Akt) activities by T. cruzi during parasite-host cell interaction. Treatment of nonphagocytic cells (Vero, L(6)E(9), and NIH 3T3) and phagocytic cells (human and J774 murine macrophages) with the selective PI3K inhibitors Wortmannin and LY294002 significantly impaired parasite invasion in a dose-dependent fashion. A strong activation of PI3K and PKB/Akt activities in Vero cells was detected when these cells were incubated with trypomastigotes or their isolated membranes. Consistently, we were unable to detect activation of PI3K or PKB/Akt activities in host cells during epimastigote (noninfective) membrane-host cell interaction. Infection of transiently transfected cells containing an inactive mutant PKB showed a significant inhibition of invasion compared with the active mutant-transfected cells. T. cruzi PI3K-like activity was also required in host cell invasion since treatment of trypomastigotes with PI3K inhibitors prior to infection reduced parasite entry. Taken together, these results indicate that PI3K and PKB/Akt activation in parasites, as in host cells induced by T. cruzi, is an early invasion signal required for successful trypomastigote internalization.     

Effects of norepinephrine or prostaglandin E2 on extracellular acidification rate of MCG 101, or K1735-M2 tumor cells

We studied by microphysiometry functional effects of two different signalling molecules in the murine tumor cell lines, MCG 101 and K1735-M2, namely norepinephrine (NE) and prostaglandin E2 (PGE2). This methodology implies estimation of intracellular metabolism by measurements of extracellular acidification rate (ECAR). MCG 101 (an undifferentiated, epithelial-like tumor), in contrast to K1735-M2 (a melanoma), has been found to produce great amounts of PGE2. Challenge of MCG 101 cells with PGE2 (0.284 and 2.84 microM for 9 min) elicited an increase in ECAR by about 10 and 41% above basal level, respectively. Pretreatment with indomethacin (0.5 microM) reduced the response to the two PGE2 concentrations by about 70 and 25%, respectively. In contrast, PGE2 caused virtually no response in K1735-M2 cells. Moreover, NE caused increases in ECAR in both cell types, possibly via beta3-adrenoceptors, as investigated pharmacologically in MCG 101, and by immunocytochemistry in both cell lines. The results obtained strongly suggest functional receptors for PGE2 in MCG 101, but not K1735-M2 tumor cells. Functional receptors for NE were demonstrated in both cell lines. There is possibly an autocrine loop in the MCG 101 cells, in which PGE2 activates cyclooxygenase.     

Fractal Organization of Cultivated in vitro Spiculogenous Cells and Larval Spicules of the Sea Urchin Strongylocentrotus nudus

The morphological patterns of the cultivated cells of primary mesenchyme and the spicules of the larval skeleton of the sea urchin Strongylocentrotus nudus were quantified, and the value of their fractal dimensions (D) was determined with ImageJ 1.20s software. It was shown that during cytodifferentiation, the values of D in the fractal (fractional) dimension, which reflects the complex spatial organization of the spiculogenous mesenchyme elements in two-dimensional space, increase to values close to 1.7. The invertible treatment with cytochalasin, which destroys the system of the actin filaments, suppresses the normal control of biomineralization and causes a complex form of spicules, the fractal dimension of which varies within 1.5–1.6. Thus, the determination of the fractal dimension value serves as evidence of the fractional essence of the patterns studied, quantifies the spatially complex organization of cells and their assemblies during morphogenesis, and allows us to estimate the variation in the spicule morphology after cytochalasin treatment.     

Fractal dimension and histogram method: Algorithm and some preliminary results of noise-like time series analysis

In the present work a methodological background for the histogram method of time series analysis is developed. Connection between shapes of smoothed histograms constructed on the basis of short segments of time series of fluctuations and the fractal dimension of the segments is studied. It is shown that the fractal dimension possesses all main properties of the histogram method. Based on it a further development of fractal dimension determination algorithm is proposed. This algorithm allows more precision determination of the fractal dimension by using the “all possible combination” method. The application of the method to noise-like time series analysis leads to results, which could be obtained earlier only by means of the histogram method based on human expert comparisons of histograms shapes.     

Plasmodium falciparum polypeptides interacting with human red cell membranes show high affinity binding to Band-3

P. falciparum proteins were labelled with [35S]methionine and harvested at various asexual stages. A number of parasite proteins bound to uninfected red cell membranes (ghosts). Some of these proteins differentially partitioned when ghosts were extracted with detergent. Several of these proteins bound very strongly to immobilised whole ghost proteins or immobilised purified Band-3 in a stage-specific manner, but not to a sham-coupled matrix or to immobilised Band-3 extract from cells rendered refractory to invasion. Such specific binding of parasite proteins to immobilised Band-3 supports recent conjecture as to its role as a host receptor during parasite invasion. However, our results demonstrate the complex and multifactorial nature of the interaction between parasite and host proteins during invasion and development.     

A fractal model for the characterization of mycelial morphology

A new technique based on a fractal model has been developed for the quantification of the macroscopic morophology of mycelia. The morphological structuring is treated as a fractal object, and the fractal dimension, determined by an ultrasonic scattering procedure developed for the purpose, serves as a quantitative morphological index. Experimental observations reported earlier and simulations of mycelial growth, carried out using a probabilistic-geometric growth model developed for the purpose, both validate the applicability of the fractal model. In experiments with three different species, the fractal dimensions of pelletous structures were found to be in the range 1.45-2.0 and those of filamentous structures were in the range 1.9-2.7, with values around 2.0 representing mixed morphologies. Fractal dimensions calculated from simulated mycelia are in rough agreement with these ranges. The fractal dimension is also found to be relatively insensitive to the biomass concentration, as seen by dilution of the original broths. The relation between morphology and filtration properties of the broths has also been studied. The fractal dimension shows a strong correlation with the index of cake compressibility and with the Kozeny constant, two filtration parameters that are known to be morphology dependent. This technique could thus be used to develop correlations between the morphology, represented by the fractal dimension, and important morphology-dependent process variables. (c) 1993 John Wiley & Sons, Inc.     

华蟾素对子宫内膜癌HEC-1-B细胞株凋亡和增殖的影响

目的：探讨华蟾素对体外培养子宫内膜癌HEC-1-B细胞凋亡、增殖以及侵袭能力的影响。方法：体外培养HEC-1-B细胞,经不同浓度华蟾素（0．2mg／ml、2mg／ml和20mg／m1）干预24h后,采用MTT法观察细胞生长情况,流式细胞术分析细胞凋亡,Transwell小室检测细胞体外侵袭能力。结果：华蟾素能有效抑制HEC．1．B细胞生长,诱导细胞凋亡。未经华蟾素处理的细胞凋亡率仅为2．5％,经0．2mg／ml、2mg／ml、20mg／ml的华蟾素作用24h后,细胞凋亡率分别为7．4％、44．3％和78．5％。趋势卡方检验x^2=165．4983,P〈0．0001。HEC-1-B细胞经华蟾素作用后,细胞侵袭能力降低。在高浓度时,华蟾素有可能存在细胞毒作用。结论：华蟾素能通过诱导HEC-1-B细胞凋亡,从而抑制HEC-1-B细胞生长,并且降低细胞的侵袭能力。