Intravesical administration of exogenous microRNA-145 as a therapy for mouse orthotopic human bladder cancer xenograft

We previously reported that the level of microRNA (miR)-145 is attenuated in human bladder cancer cells. In this current study, we investigated whether intravesical administration of miR-145 could be a potential therapeutic strategy for controlling bladder cancer by using an orthotopic human bladder cancer xenograft model. Following transfection of 253J B-V cells with miR-145, the effects of the ectopic expression of miR-145 were examined by performing MTT, Western blotting analysis, Hoechst33342 staining, and wound healing assay in vitro. Also, a mouse orthotopic human bladder cancer model was established by inoculating 253J B-V cells into the bladder wall of mice. The anti-cancer effects of intravesical injections of miR-145 into these mice were then assessed. Transfection of 253J B-V cells with miR-145 induced apoptosis and suppression of cell migration in vitro. Western blotting showed that the levels of c-Myc, socs7, FSCN1, E-cadherin, β-catenin, and catenin δ-1 were decreased and that the PI3K/Akt and Erk1/2 signaling pathways were increased in compensatory fashion. In vivo, mice treated with miR-145 showed 76% inhibition of tumor growth, with a significant prolongation of animal survival (p = 0.0183 vs. control). Western blotting showed that both apoptosis and cell motility-related genes were significantly decreased as seen in vitro. Furthermore, PI3k/Akt and Erk1/2 signaling pathways, which were activated in a compensatory manner in vitro, were decreased in vivo. Intravesical administration of exogenous miR-145 was thus concluded to be a valid therapy for bladder cancer in this human bladder cancer xenograft model.     

Herpes Simplex Encephalitis: A light and electron microscopic study in a fatal case

A fatal case was described of a 41–year-old woman with a tentative clinical diagnosis of acute viral meningoencephalitis of nine days' duration. The neuropathologic findings by light microscopy resembled those of acute necrotizing encephalitis or herpes simplex encephalitis, including eosinophilic intranuclear inclusion bodies of Cowdry type A. Electron microscopic study of these inclusions demonstrated the presence of herpes-type virus particles. Though the titer of herpes simplex virus examined on the sixth day of the illness was not elevated and the isolation of the virus was not successful, the case was regarded as herpes simplex encephalitis clinicopatholo-gically.     

Biochemical and immunohistochemical studies on carcinoembryonic antigen of ovarian mucinous and serous tumors

The carcinoembryonic antigen (CEA) in the cyst fluid of ovarian mucinous and serous tumors was investigated. The molecular weight and antigenicity of the CEA from both ovarian tumors were very similar to those of colon cancer CEA as determined by SDS electrophoresis and double immunodiffusion on agar plates. In the cyst fluid of ovarian mucinous tumors, the amount of CEA was generally high and CEA of molecular weight (MW) 200,000 was increased. In contrast, in the cyst fluid of ovarian serous tumors, the CEA amount was low and CEA variants of MW 370,000 and 180,000 were present in addition to the main CEA of MW 200,000. Immunohistochemically, CEA was stained mainly in the intestinal type epithelium of ovarian mucinous tumors, and the CEA revealed a tendency to be stained more frequently and strongly with increasing degree of tumor malignancy. Thus, ovarian mucinous tumors (especially the intestinal type epithelium) produced large amounts of CEA which closely resembled colon cancer CEA, whereas ovarian serous tumors produced small amounts of CEA, including some CEA variants. In the study of ovarian epithelial tumors, CEA may be useful as a marker for the malignant transformation of ovarian mucinous tumors.     

In vivo treatment of mutant FLT3-transformed murine leukemia with a tyrosine kinase inhibitor.

Somatic mutation of the FLT3 gene, in which the juxtamembrane domain has an internal tandem duplication, is found in 20% of human acute myeloid leukemias and causes constitutive tyrosine phosphorylation of the products. In this study, we observed that the transfection of mutant FLT3 gene into an IL3-dependent murine cell line, 32D, abrogated the IL3-dependency. Subcutaneous injection of the transformed 32D cells caused leukemia in addition to subcutaneous tumors in C3H/HeJ mice. To develop a FLT3-targeted therapy, we examined tyrosine kinase inhibitors for in vitro growth suppression of the transformed 32D cells. A tyrosine kinase inhibitor, herbimycin A, remarkably inhibited the growth of the transformed 32D cells at 0.1 microM, at which concentration it was ineffective in parental 32D cells. Herbimycin A suppressed the constitutive tyrosine phosphorylation of the mutant FLT3 but not the phosphorylation of the ligand-stimulated wild-type FLT3. In mice transplanted with the transformed 32D cells, the administration of herbimycin A prolonged the latency of disease or completely prevented leukemia, depending on the number of cells inoculated and schedule of drug administration. These results suggest that mutant FLT3 is a promising target for tyrosine kinase inhibitors in the treatment of leukemia.     

Visualization of flow resistance in physiological nasal respiration: analysis of velocity and vorticities using numerical simulation

OBJECTIVES: To visualize the velocity gradients and the vorticities of physiological unsteady nasal flow using the computational fluid dynamics method and to compare the inspiratory phase and expiratory phase flow patterns. DESIGN: An anatomically correct 3-dimensional nasal and pharyngeal cavity was constructed from computed tomographic images of a healthy adult nose and pharynx. The unsteady state Navier-Stokes and continuity equations were solved numerically on inspiratory and expiratory nasal flow. SETTING: Numerical simulation application. PARTICIPANTS: Coronary and axial computed tomographic images from a healthy adult were used. MAIN OUTCOME MEASURES: The detailed velocity distribution and vorticity (resistance) distribution of nasal airflow were visualized using the computational fluid dynamics method (an imaging technology for regional flow factors [velocity, vector, streamline, and vortex]). RESULTS: In the inspiratory phase, a high-velocity area was prominent in the middle meatus, and the highest vorticity area had good agreement with this region. In the expiratory phase, the distributions of velocity and vorticities were flatter than those in the inspiratory phase. CONCLUSION: The computational fluid dynamics model allows the investigation of airflow elements under physiological conditions, as well as the examination of the effect of nasal structure.     

Growth Characteristics of Retinal Capillary Endothelial Cells Compared with Pulmonary Vein Endothelial Cells in Culture

Bovine retinal capillary endothelial cells (RCECs) and pulmonary vein endothelial cells (PVECs) were isolated and investigated in plate culture, three-dimensional culture and in co-culture with pericytes. In plate culture, RCECs required growth factor in the medium for growth whereas PVECs did not. Phenotypic modulation (a tendency to become similar morphologically to smooth muscle cells, and to accumulate into thread-like structures) was observed in PVECs but not in RCECs. In three-dimensional culture, RCECs contracted, aggregated and were unable to proliferate. Proliferation was elicited when the gel matrix was adsorbed by fibronectin or upon co-culture with pericytes. In contrast, PVECs not only proliferated but also formed tubular structures. In co-culture with pericytes, PVECs in close contact with, or in near apposition to pericytes formed tubular structures earlier than those without contact in the same dish. These results provide new findings about differences in the growth characteristics of endothelial cells between microvessels and large vessels. In addition, it is considered that pericytes may promote tube formation by endothelial cells in three-dimensional culture. Acta Pathol Jpn 41: 133-142, 1991.     

ONTOGENY OF HEPATIC FATTY ACID-BINDING PROTEIN IMMUNOREACTIVITY IN HUMAN LIVER and INTESTINAL TRACT

Liver and intestinal tissues of human fetuses at gestational ages between 6 and 30 weeks were immunostained with rabbit antibody against fatty acid-binding protein (FABP) isolated from rat liver, since the antibody crossreacted with human FABP of the hepatic type. FABP-immunoreactive hepatocytes were found in the liver as early as the 7th week of gestation, but not at the 6th week. The frequency of immunoreactive cells was about 80% throughout the gestational period examined. No immunoreactive cells other than hepatocytes were found in liver tissue. In the intestinal tract, ileal, colonic and vermiform appendicular FABP immunoreactivity was demonstrated at the 23rd week of gestation, and duodenal and jejunal immunoreactivity at the 26th week. Positive cells in the jejunum were very few at this stage, but numerous at the 30th week of gestation. The immunoreactive cells were primitive absorptive cells in intestinal villi, and no cryptic epithelial cells were positively immunostained. Thus, FABP immunoreactivity was considered to be a marker for hepatocytes at the early to late fetal stage, and for intestinal absorptive cells at mid- to late fetal stage. ACTA PATHOL JPN 38: 979∼987, 1988.     

Effects of estrus cycle on thermoregulatory responses during exercise in rats

Summary In female rats, rectal temperature (T _re), tail vasomotor response, oxygen uptake , and carbon dioxide production were measured in proestrus and estrus stages during treadmill running at two different speeds at an ambient temperature (T _a) of 24° C. Experiments were performed at 2.00–6.00 a.m., when the difference inT _re was greatest between the two stages;T _re at rest in the estrus stage was 0.54° C higher than in the proestrus stage. In a mild warm environment, thresholdT _re for a rise in tail skin temperature (T _tail) was also higher in the estrus stage than in the proestrus stage. In contrast, no difference was seen in the thresholdT _re and steady stateT _re at the end of exercise between proestrus and estrus stages. These values were higher at the higher work intensity. was also similar between the two stages, except in the second 5 min after the beginning of exercise, when was greater andT _re rose more steeply in the proestrus stage. These data indicate that deep body temperature during exercise is regulated at a certain level depending on the work intensity and is not influenced by the estrus cycle.This study was supported in part by a Grant-in Aid for Scientific Research from the Ministry of Education, Science and Culture of Japan (Grant No. 62480114)     

Cell Cycle Regulation and Differentiation in the Human Podocyte Lineage

Mature podocytes are regarded as growth-arrested cells with characteristic phenotypic features that underlie their function. To determine the relationship between cell cycle regulation and differentiation, the spatiotemporal expression of cyclin A, cyclin B1, cyclin D1, the cyclin-dependent kinase inhibitors (CKIs) p27 and p57, and markers of differentiating podocytes in developing human kidneys was investigated by immunohistochemistry. In S-shaped body stage, Ki-67, a cell proliferation marker that labels the G1/S/G2/M phase, was expressed in the majority (more than 80%) of presumptive podocytes, along with cyclin A (~20% of the Ki-67-positive cells) and cyclin B1 (less than 5% of Ki-67-positive cells) expression. Among these cells, cyclin D1 and CKIs were markedly down-regulated. At the capillary-loop stage, by contrast, CKIs and cyclin D1 were intensely positive in podocytes, whereas no Ki-67, cyclin B1, or cyclin A expression was seen. Moreover, double-immunolabeling and serial-section analysis provided evidence that CKIs and markers specific for differentiating podocytes, namely PHM-5 (podocalyxin-like protein in humans), synaptopodin (a foot process-related protein), and C3b receptor, were co-expressed at the capillary-loop stage. Podocytes were the only cells within the glomeruli that expressed CKIs at immunohistochemically detectable levels. Furthermore, bcl-2 (an apoptosis inhibitory protein) showed a reciprocal expression pattern to that of CKI. These results suggest that 1) the cell cycle of podocytes is regulated by cyclin and CKIs, 2) CKIs may act to arrest the cell cycle in podocytes at the capillary-loop stage, and 3) the specific cell cycle system in podocytes may be closely correlated with their terminal differentiation in humans.