Changes in the mitotic activity of the corneal epithelium of white rats following coolong of the animals at different times of the day]

A study was made of the influence of moderate hypothermia on the mitotic activity of albino rat corneal epithelium. The animals were cooled by the contact method for one hour to 28 degrees C; such procedure was conducted at 6 a.m., at noon, and at 6 p.m.; the epithelial reaction to cooling proved to depend on the time, the greatest suppression of mitotic activity (14-fold) occurring at daytime 3 hours after the cooling. A tendency to normalization of cell division was observed 6 and 12 hours after the cooling. The number of mitoses decreased 3 hours after the evening cooling, no changes in the mitotic activity in 3 and 6 hours after the morning cooling; cell division was found to be suppressed in 12 hours.     

Changes in the proliferative activity of the corneal epithelium and the regenerating liver in partial splenectomy in mice

The mitotic activity in epithelial cells of the mouse cornea was studied 4 h, 1, 2, 5, 8 and 14 days after a sham operation or partial (2/3) splenectomy. The decrease in the number of dividing cells in the corneal epithelium was observed within two days after a sham operation and within five days after partial splenectomy. On the contrary, partial hepatectomy increased the number of mitoses in the corneal epithelium. Liver regeneration against the background of a sham operation or partial splenectomy was accompanied by a lesser number of mitoses (by a factor of 2.5-4) in hepatocytes than in the animals subjected to partial hepatectomy only.     

Rabbits' corneal cells studied in tissue cultures

Summary Enzymatic reactions of corneal epithelial cells are, by and large, stronger than reactions of corneal fibroblasts.The cytoplasm of corneal epithelial cells and fibroblasts has stronger enzymatic activity than the nuclei of the two types of cells.The nuclei of epithelial cells react stronger than the nuclei of fibroblasts.Certain enzymes have a fairly characteristic cytoplasmic distribution in corneal epithelial cells but not in fibroblasts. The intensity of some enzyme reactions changes with aging of the cells.This study was aided in part by an institutional grant from the Lilly Research Laboratories, Indianapolis, Ind.     

人胚胎角膜上皮细胞系的建立和生物学特性

为构建角膜基础研究的稳定载体和操作平台,通过合法渠道获得人胚胎,并对角膜上皮细胞进行了分离培养。经反复传代,初步建立了人胚胎角膜上皮细胞系,并对其生物学特性进行了研究。结果显示,培养细胞具有较典型的上皮细胞特征。细胞生长较快,最快时两天可传代一次。K19和PCNA在各代胚胎角膜细胞均有表达,K19的表达部位位于胞浆,而PCNA的表达部位位于胞核。处于细胞周期中S期的细胞比例大约为11%￣23%。染色体核型分析表明各代细胞染色体的数目和形态相似。因此,人胚胎角膜上皮细胞适合于建立相对稳定的细胞系。培养细胞具有分化上的幼稚性和较强且稳定的增殖能力,细胞生长状态良好,而且该细胞系的遗传特征较为稳定。     

The Corneal Epithelium as A Source of Mammalian Somatic Mitoses

Dividing cells that occur abundantly in the lowermost layers of the corneal epithelium of various laboratory mammals provide a reliable and readily procurable source of mitotic figures for studies of chromosome number and form. Preparations may be secured quickly by fixing and staining entire eyes in an orcein-alcohol-acetic-acid mixture, or by fixing in acetic-alcohol and then staining with orcein or with leucobasic f uchsin as used in the Feulgen technic. For cytological examination of the epithelial cells and for determination of mitotic rates, the cornea is dissected from the eye and mounted as a flat preparation. Squashes of the epithelial cells are useful if mitotic counts are not required.     

Activation of cell division and nucleic acid synthesis in the corneal epithelium of white rats undergoing repeated exposure to stress

A study was made of the influence of single and repeated stress on the mitotic activity and synthesis of DNA and RNA in the corneal epithelium of albino rats. The stressors used were fixation on the back during one hour, the influence of 1.5-h hyperthermia (41.5 degrees C), and the influence of hypoxia (4h, 9000 m). Single stress induced the depression of the mitotic activity. The autography tests of DNA synthesis were made constantly. Repeated stress (5 exposures) entailed activation of the synthesis of the nucleic acids and cell division, evidence of a structural trace of stress, in the epithelial tissues.     

Correlation between tissue growth kinetics and modulation of mouse skin tumorigenesis by phorbol esters.

Previous studies on the influence of phorbol esters on mouse skin tumorigenesis have shown that 12-O-tetradecanoylphorbol-13-acetate (TPA) enhances development of malignant epithelial and mesenchymal skin tumors by a completely carcinogenic dose of 3-methylcholanthrene (MCA), while its congener phorbol-12, 13-diacetate (PDA) exerts an inhibitory effect. Differential effects of these two agents were analysed by histology, morphometry and cell kinetic techniques including autoradiography and estimation of labelled precursor incorporation into DNA by liquid scintillation counting. Epidermal hyperplasia induced on exposure of S/RV Cri mouse skin to a single or multiple TPA application after MCA injection was associated with a significant increase in the thickness of nucleated cell layers, stratum granulosum, number of suprabasal cells and dark basal cells. Enhancing effect of TPA on MCA-induced neoplastic development correlated well with an increase in mitotic activity, number of cells in S-phase and increased rate of DNA synthesis in the epidermis, dermis and subcutis as also mast cell number. In contrast, treatment of MCA-injected preneoplastic mouse skin with PDA resulted in epidermal hypoplasia and cellular damage evident as cytoplasmic vacuolation and nuclear pyknosis. Multiple PDA exposure also reduced the thickness, mitotic index and number of cells in S-phase in epidermis, dermis and subcutis. Thus, cellular toxicity and inability to recruit cells in DNA-synthetic phase may account for inhibition of progression of preneoplastic epithelial and mesenchymal cells into overt tumors by PDA.     

Cell proliferation in mouse tissues after thymectomy and the administration of T-activin

The epithelium of mouse cornea and lymph nodes was examined for DNA-synthetic and mitotic activity at different times after thymectomy and administration of T-activin, an active factor of the thymus. Thymectomy entails retardation of the rate of corneal epithelium regeneration, diminution in both tissues under study of the amplitude of oscillations in cell proliferation throughout the day. Administration to the animals of the immunoactive thymic factor T-activin makes the circadian rhythm of cell proliferation return to normal. It is assumed that T-activin raises the capacity of lymphocytes to interact with epithelial cells, which manifests itself in the enhancement of their mitotic activity.     

Evidence for the presence of inhibitors of mitotic factors during G1 period in mammalian cells

Our earlier studies indicated that the mitotic factors, which induce germinal vesicle breakdown and chromosome condensation when injected into fully grown Xenopus oocytes, are preferentially associated with metaphase chromosomes and that they bind to chromatin as soon as they are synthesized during the G2 phase. In this study, we attempted to determine the fate of these factors as the cell completes mitosis and enters G1. Extracts from HeLa cells at different points during G1, S, and G2 periods were mixed with mitotic extracts in various proportions, incubated, and then injected into Xenopus oocytes to determine their maturation-promoting activity. The maturation-promoting activity of the mitotic extracts was neutralized by extracts of G1 cells during all stages of G1 but not by those of late S and G2 phase cells. Extracts of quiescent (G0) human diploid fibroblasts exhibited very little inhibitory activity. However, UV irradiation of G0 cells, which is known to cause decondensation of chromatin, significantly enhanced the inhibitory activity of extracts of these cells. These factors are termed inhibitors of mitotic factors (IMF). They seem to be activated, rather than newly synthesized, as the cell enters telophase when chromosomes begin to decondense. The IMF are nondialyzable, nonhistone proteins with a molecular weight of greater than 12,000. Since mitotic factors are known to induce chromosome condensation, it is possible that IMF, which are antagonistic to mitotic factors, may serve the reverse function of the mitotic factors, i.e., regulation of chromosome decondensation.     

Antagonistic effect of selenite on tumor promoter induced cell proliferation in cultures of rat tongue epithelium

In cultures of rat tongue epithelial cells, cell proliferation following incubation with different doses of the potent tumor promoter TPA has been studied by using a stathmokinetic method counting colchicine arrested metaphases. It was demonstrated that 24 h incubation with concentrations higher than 5 ng TPA/mL medium caused inhibition, whereas below 5 ng TPA/mL medium caused stimulation of the mitotic activity reaching a maximum around 30 h from the start of the incubation period. Based on the evidence of the anticarcinogenic effect of selenium in several animal models, experiments have been performed elucidating the influence of an atoxic dose (1/1.000.000M) of selenite on the observed TPA-induced cell proliferation. Our results indicate that addition to the culture medium of an atoxic dose of selenite, not affecting the mitotic activity of control cultures, inhibits the TPA-induced stimulation of cell proliferation.     

Myelokaryocyte mitotic activity during microwave irradiation (2375 MHz)

Changes in mitotic activity of myelocaryocytes exposed to super-high frequency field (2375 MHz) of 10, 50 and 500 microW/cm2 for a month show the influence of this factor on the DNA synthesis, premitotic processes and cell reproduction biorhythms depending on the radiation intensity.     

Selective effect of fractions of a yeast extract (PCO) on normal and malignant cells

The selective action of two fractions of PCO (a yeast extract) on normal and malignant cells was demonstrated. In vivo, the mitotic activity of malignant cells was inhibited by the methanol-insoluble fraction of PCO, whereas the methanol-soluble fraction caused no inhibition. The in vitro studies, however, showed inhibition of mitoses with both fractions. The malignant cells employed in vitro and in vivo were the Krebs-2 and Ehrlich carcinomas. The nonneoplastic cells tested in vitro were established cultures of epithelial-like cells from murine bone marrow and thymus, and corneal epithelium and peripheral blood in vivo.     

Proliferative reaction of the epithelium of gastric glands to vagotomy and sympathectomy

By means of autoradiography and metaphase arrest technique 24-hour rhythms and intensity of proliferative processes in the epithelium of gastric glands were studied, as well as morphometric status of these structures after vagotomy and drug sympathectomy in the rat. In both cases the reaction of glandular epithelium appeared with the increase of mitotic activity and the decrease of cell synchronization before the entry into DNA--synthesis and mitosis. The number of epithelial cells in gastric glands became reduced, but after vagotomy, unlike sympathectomy, mainly because of the lack of chief cells. Thus, the trophic control upon the dynamic structure of gastric glands may have different mechanisms of realization for parasympathetic and sympathetic nervous system, probably, through the influence on cell proliferation or differentiation.     

Symmetric and asymmetric cell division in rat corneal epithelium

Mitotic cells in normal, mature rat corneal epithelium were examined with a light microscope on serial, semi-thick plastic sections. Classification of mitotic figures into horizontally, obliquely or vertically positioned with reference to the epithelial basal lamina has shown that no single configuration predominates. A striking correlation between the position of the daughter cells after cytokinesis and their morphology has been observed. Horizontal cytokinetic pairs were morphologically symmetric but vertical ones were asymmetric, displaying distinct differences between daughter cells. Analysis of earlier mitotic phases has shown that the asymmetry could also be observed in vertical anaphases and telophases. The data provide clear morphological evidence for real asymmetric (unequal) cell division in a replacing epithelium in an adult mammal. It is concluded that asymmetric cell division in the corneal epithelium coexists with, and is as frequent as symmetric (equal) cell division. Randomness of mitotic spindle positioning implies that diverse forms of cell transfer from the proliferative into the differentiative epithelial compartments must operate. Therefore, the universality of the general model of cell renewal in stratified epithelia, which assumes a strong predominance of horizontal mitoses, exclusively equal mitotic divisions and one form of cell transfer, is questioned.     

CDK5 regulates cell adhesion and migration in corneal epithelial cells

CDK5 and its activator, p35, are expressed in mouse corneal epithelium and can be coimmunoprecipited from corneal epithelial cell lysates. Immunostaining shows CDK5 and p35 in all layers of the corneal epithelium, especially along the basal side of the basal cells. Stable transfection of corneal epithelial cells with CDK5, which increases CDK5 kinase activity by approximately 33%, also increases the number of cells adhering to fibronectin and the strength of adhesion. CDK5 kinase activity seems to be required for this effect, because the kinase inactive mutation, CDK5-T33, either reduces adhesion or has no significant effect, depending on the level of expression. Using an in vitro scrape wound in confluent cultures of stably transfected cells to examine the effect of CDK5 on cell migration, we show that reoccupation of the wound area is significantly decreased by CDK5 and increased by CDK5-T33. These findings indicate that CDK5 may be an important regulator of adhesion and migration of corneal epithelial cells.     

Symmetric and asymmetric cell division in rat corneal epithelium

Abstract. Mitotic cells in normal, mature rat corneal epithelium were examined with a light microscope on serial, semi-thick plastic sections.
Classification of mitotic figures into horizontally, obliquely or vertically positioned with reference to the epithelial basal lamina has shown that no single configuration predominates. A striking correlation between the position of the daughter cells after cytokinesis and their morphology has been observed. Horizontal cytokinetic pairs were morphologically symmetric but vertical ones were asymmetric, displaying distinct differences between daughter cells. Analysis of earlier mitotic phases has shown that the asymmetry could also be observed in vertical anaphases and telophases.
The data provide clear morphological evidence for real asymmetric (unequal) cell division in a replacing epithelium in an adult mammal. It is concluded that asymmetric cell division in the corneal epithelium coexists with, and is as frequent as symmetric (equal) cell division. Randomness of mitotic spindle positioning implies that diverse forms of cell transfer from the proliferative into the differentiative epithelial compartments must operate. Therefore, the universality of the general model of cell renewal in stratified epithelia, which assumes a strong predominance of horizontal mitoses, exclusively equal mitotic divisions and one form of cell transfer, is questioned.     

Ultrastructural and autoradiographic observations of hamster cheek pouch epithelium grown in vitro

Summary Epithelial outgrowths from hamster cheek pouch explants were cultured for varying peroids of time up to 22 days. Growth of the epithelial sheets was monitored, employing colcemid for demonstrating mitotic activity and tritiated thymidine for DNA synthesis. Mitoses and thymidine uptake were observed among epithelial outgrowths at a considerable distance from the original explant. The epithelial nature of the growing cell sheets was confirmed, employing electron microscopic techniques. The cells exhibited the presence of tonofilaments, desmosomes, ribosomes, Golgi, mitochondria, and rough endoplasmic reticulum. The cultured explants were treated with cyclic nucleotides in order to investigate their modulatory effects on epithelial cell differentiation. Dibutyryl cAMP induced marked mitotic inhibition (46.3%) in our assay, which was increased to 57% with the addition of theophylline. Dibutyryl cGMP showed only a mild (5%) stimulatory effect on mitotic activity. Dibutyryl cAMP enhanced keratinization in the epithelial cell out-growths with the biogenesis of keratohyalin granules, whereas dibutyryl cGMP did not produce any observable alterations.     

Knockdown of heme oxygenase-2 impairs corneal epithelial cell wound healing

Heme oxygenase (HO) represents an intrinsic cytoprotective system based on its anti‐oxidative and anti‐inflammatory properties mediated via its products biliverdin/bilirubin and carbon monoxide (CO). We showed that deletion of HO‐2 results in impaired corneal wound healing with associated chronic inflammatory complications. This study was undertaken to examine the role of HO activity and the contribution of HO‐1 and HO‐2 to corneal wound healing in an in vitro epithelial scratch injury model. A scratch wound model was established using human corneal epithelial (HCE) cells. These cells expressed both HO‐1 and HO‐2 proteins. Injury elicited a rapid and transient increase in HO‐1 and HO activity; HO‐2 expression was unchanged. Treatment with biliverdin or CORM‐A1, a CO donor, accelerated wound closure by 10% at 24 h. Inhibition of HO activity impaired wound closure by more than 50%. However, addition of biliverdin or CORM‐A1 reversed the effect of HO inhibition on wound healing. Moreover, knockdown of HO‐2 expression, but not HO‐1, significantly impaired wound healing. These results indicate that HO activity is required for corneal epithelial cell migration. Inhibition of HO activity impairs wound healing while amplification of its activity restores and accelerates healing. Importantly, HO‐2, which is highly expressed in the corneal epithelium, appears to be critical for the wound healing process in the cornea. The mechanisms by which it contributes to cell migration in response to injury may reside in the cytoprotective properties of CO and biliverdin. J. Cell. Physiol. 226: 1732–1740, 2011. © 2010 Wiley‐Liss, Inc.     

Ultrastructural and autoradiographic observations of hamster cheek pouch epithelium grown in vitro.

Epithelial outgrowths from hamster cheek pouch explants were cultured for varying periods of time up to 22 days. Growth of the epithelial sheets was monitored, employing colcemid for demonstrating mitotic activity and tritiated thymidine for DNA synthesis. Mitoses and thymidine uptake were observed among epithelial outgrowths at a considerable distance form the original explant. The epithelial nature of the growing cell sheets was confirmed, employing electron microscopic techniques. The cells exhibited the presence of tonofilaments, desmosomes, ribosomes, Golgi, mitochondria, and rough endoplasmic reticulum. The cultured explants were treated with cyclic nucleotides in order to investigate their modulatory effects on epithelial cell differentiation. Dibutyryl cAMP induced marked mitotic inhibition (46.3%) in our assay, which was increased to 57% with the addition of theophylline. Dibutyryl cGMP showed only a mild (5%) stimulatory effect on mitotic activity. Dibutyryl cAMP enhanced keratinization in the epithelial cell outgrowths with the biogenesis of keratohyalin granules, whereas dibutyryl cGMP did not produce any observable alterations.     

Mitotic activity changes in the corneal epithelium of rats of different ages following exposure to pain]

A study was made of pain stimulus (amputation of 1/3 of the tail) on the mitotic activity in the corneal epithelium of 21-day fetuses, 1-, 3-, 4-, 5-, 7-, 10-, 15-, 20- and 25-day rats. In 45 minutes after the infliction of trauma no significant change was seen in the cornea of the fetuses and of the one-day-old ratlings. A gradual establishment of the reactive inhibition of mitoses in response to pain occurred between the 3rd and the 10th day of postnatal development. This reaction became more intense after the 10th day, reaching the maximum by the 25th day. Reactive inhibition of the mitotic activity was connected with the inhibition of the entrance of cells into mitosis.