A pituitary-salivary mixed gland induced by tissue recombination of embryonic pituitary epithelium and embryonic submandibular gland mesenchyme in mice

Renal subcapsular syngrafts of Day 9 to 11 mouse embryonic pituitary epithelium with Day 14 mouse embryonic submandibular gland mesenchyme produced mixed organs that include residual cleft structure surrounded by anterior pituitary cells some which are stained by anti-ACTH antiserum and submandibular gland-like structure with differentiated acinar cells which are stained by anti-alpha-amylase antiserum. However, when Day 8.5 or 12 embryonic pituitary epithelium was recombined with submandibular gland mesenchyme and syngrafted, development of submandibular gland-like or anterior pituitary tissues resulted, respectively. Thus, during organogenesis of the mouse anterior pituitary, there exists a developmental stage (Day 8.5-11 in utero), when prospective pituitary epithelium can respond to heterotypic submandibular gland mesenchyme with the development of a submandibular gland-like tissue.     

IL-26 mediates epidermal growth factor receptor-tyrosine kinase inhibitor resistance through endoplasmic reticulum stress signaling pathway in triple-negative breast cancer cells

Triple-negative breast cancer (TNBC) has a poor prognosis compared to other breast cancer subtypes. Although epidermal growth factor receptor (EGFR) is overexpressed in TNBC, clinical trials with EGFR inhibitors including tyrosine kinase inhibitors (EGFR-TKI) in TNBC have heretofore been unsuccessful. To develop effective EGFR-targeted therapy for TNBC, the precise mechanisms of EGFR-TKI resistance in TNBC need to be elucidated. In this study, to understand the molecular mechanisms involved in the differences in EGFR-TKI efficacy on TNBC between human and mouse, we focused on the effect of IL-26, which is absent in mice. In vitro analysis showed that IL-26 activated AKT and JNK signaling of bypass pathway of EGFR-TKI in both murine and human TNBC cells. We next investigated the mechanisms involved in IL-26-mediated EGFR-TKI resistance in TNBC. We identified EphA3 as a novel functional receptor for IL-26 in TNBC. IL-26 induced dephosphorylation and downmodulation of EphA3 in TNBC, which resulted in increased phosphorylation of AKT and JNK against EGFR-TKI-induced endoplasmic reticulum (ER) stress, leading to tumor growth. Meanwhile, the blockade of IL-26 overcame EGFR-TKI resistance in TNBC. Since the gene encoding IL-26 is absent in mice, we utilized human IL-26 transgenic (hIL-26Tg) mice as a tumor-bearing murine model to characterize the role of IL-26 in the differential effect of EGFR-TKI in human and mice and to confirm our in vitro findings. Our findings indicate that IL-26 activates the bypass pathway of EGFR-TKI, while blockade of IL-26 overcomes EGFR-TKI resistance in TNBC via enhancement of ER stress signaling. Our work provides novel insights into the mechanisms of EGFR-TKI resistance in TNBC via interaction of IL-26 with its newly identified receptor EphA3, while also suggesting IL-26 as a possible therapeutic target in TNBC.Subject terms: Stress signalling, Cell death and immune response, Breast cancer     

Existence of Two Types of Electrostatic Interaction in Reactions Catalyzed by Ferredoxin-NADP$ Oxidoreductase

Effects of salt and pH on diaphorase and NADP^$ photoreductionactivities were studied with broken spinach chloroplasts andpurified ferredoxin-NADP^$ oxidoreductase. Two types of electrostatic interactions, which regulate thereaction rate, were observed. One is the long-range electrostaticinteraction which determines the local concentrations of reactantsin the surface-mediated processes due to the change in the surfacepotential. In addition to the salt-induced change in the reactionrate, the pH optimum shift by salt was also remarkable: theoptimum pH in the diaphorase activity of chloroplasts shiftedto the more acidic pH region with an increase of salt concentration,while that of the membrane-free enzyme was not affected by salts. A more specific, short-range electrostatic interaction in reactionsbetween NADP(H) and ferredoxin-NADP^$ oxidoreductase was observed.This interaction became clearer when fixed charges on the membranesurface were masked by an addition of salts. Complete dissociationof the 2'-phosphate group of NADP(H) was necessary for its associationwith the enzyme. The eletrostatic attraction between the negativelychargedpart of NADPH and the positively-charged part of the enzyme(probably lysyl and arginyl residues) may play a role in theshort-range interaction. ¹Present address: Department of Agronomy, University of Kentucky,Lexington, Kentucky 40546, U.S.A. ²Present address: National Institute for Basic Biology, Okazaki444, Japan. (Received February 21, 1983; Accepted March 17, 1984)     

Organ specific expression of ras oncoproteins during growth and development of the rat

Summary Expression of proteins encoded by the ras proto-oncogenes was examined in extracts from normal rat organs using anti-ras p21 antibodies generated against synthetic peptides. The highest level of ras p21 was found in brain (cerebrum) and was predominantly of c-Ha-ras origin. Levels of brain ras p21 did not vary from the newborn period of 3 months of age. Moderate levels of ras p21s were detected in lung, spleen and thymus. In contrast to the p21 in brain, these levels varied with the age of the rats and were encoded by other members of ras proto-oncogene family (Ki-ras or N-ras). This organ specific expression of different ras genes might be related to developmental control of gene expressions.     

Regulation of Polyphosphoinositide Metabolism in Pea Plasma Membranes by Elicitor and Suppressor from a Pea Pathogen, Mycosphaerella pinodes

Effects of the elicitor and the suppressor from a pea pathogen,Mycosphaerella pinodes, on polyphosphoinositide metabolism inpea plasma membranes were examined in vitro. Lipid phosphorylationin the isolated pea plasma membrane was drastically stimulatedby the elicitor, but markedly inhibited by the suppressor. Asimilar inhibitory effect was observed by the treatment withorthovanadate or K-252a that blocked pisatin production inducedby the elicitor. Neomycin, an aminoglycoside antibiotic thatinteracts with the polyphosphoinositide metabolism, also affectedthe lipid phosphorylation in vitro and blocked the elicitor-inducedaccumulation of pisatin in vivo. These results suggest thatrapid changes of polyphosphoinositide metabolism in pea plasmamembranes is one of indispensable processes during the elicitationof defense responses. (Received January 22, 1992; Accepted March 23, 1992)     

The effect of prednisolone and metyrapone on FSH release induced by the administration of LRH.

The response of follicle-stimulating hormone (FSH) to a single injection of synthetic LRH was established in 7 and 6 women following an intramuscular dose of 0.2 mg and 0.1 mg. The secretion of FSH was greater in the group injected with 0.2 mg LRH than in the group injected with 0.1 mg. On the other hand, the response of FSH to a single injection of LRH (0.1 mg/subject) was established in 7 men before and after the pretreatment with metyrapone for one dat (4.5 g/subject). Pretreatment with metyrapone provoked a hypersecretion of FSH following a single injection of synthetic LRH. Seven women, 21--48 years of age who were treated with prednisolone for at least 1.5 months were examined for the responsiveness of the anterior pituitary to a single injection of synthetic LRH (0.2 MG). The secretion of FSH was not suppressed and the maximal serum level of FSH was observed 60 min after LRH injection.     

Onset and development of cannibalistic behaviour in early life stages of yellowtail

The onset and development of cannibalistic behaviour were observed in early life stages of yellowtail Seriola quinqueradiata . Cannibalistic behaviour was divided into four actions, i.e aim, chase, nip and ingestion. The frequency of chase was used as an index of cannibalistic behaviour because it always appeared in every sequence of cannibalism, although a sequence of cannibalistic behaviour sometimes stopped before nip or ingestion. No cannibalistic behaviour was observed during the larval phase until day 22 after hatching (when fish were 9.6mm T.L.) either in a rearing pond or in experimental tanks. The onset of cannibalistic behaviour was observed on day 23, coinciding with metamorphosis from the larval to juvenile phase, and it developed until day 39, with a tentative decrease between day 33 and day 36. This inverted peak corresponded roughly to the development of schooling behaviour after day 33, which was determined by distance to the nearest neighbour. In the rearing pond, suffocation of a cannibal by its prey, appeared from day 23. Field observation of juvenile yellowtails aggregating around floating seaweeds showed that cannibalism occurred in three out of 10 schools, in which six cannibals were found among 194 fish. Cannibalistic behaviour in early life stages of yellowtail may occur as a final phase of inter-individual interference and may have a role for size selection of a School member.     

Isolation of a cytotoxin from L-form Salmonella typhimurium

Abstract A cytotoxin protein was isolated from the sodium dodecyl sulphate (SDS)-solubilized extract of the stable L forms of Salmonella typhimurium by ion-retardation chromatography, ion-exchange chromatography, isoelectric focusing and gel filtration. The purified toxin, with a molecular mass of 32 kDa and with isoelectric point of 6.4, was thermolabile and trypsin-sensitive. Against mouse macrophages, its cytolytic effect was detectable in vitro at concentrations higher than 0.7 μg/ml, with a complete lysis obtained at 5 μg/ml. In contrast, it stimulated C3H/HeJ macrophages in the dose range of 0.1–0.5 μg/ml to allow the cell to respond to endotoxin, resulting in the significant production of tumor necrosis factor α. By Northern blot analysis, this effect was detectable at a dose as low as 0.01 μg/ml. These findings suggest that the transformation of bacillary S. typhimurium into L forms in vivo may induce alterations in host resistance against murine typhoid.     

Enzymatic Treatment to Eliminate the Extracellular ATP for Improving the Detectability of Bacterial Intracellular ATP

A novel and effective treatment of biological samples with a combination of adenosine phosphate deaminase and apyrase was developed for reducing extracellular ATP, which has been a major problem encountered in improving the sensitivity of assays for intracellular ATP by the firefly luciferin–luciferase (L-L) method. Under the enzymatic reaction conditions, ATP and the related adenosine derivatives were converted to IMP, which are not active to the L-L system. In the model system (3.2 × 10⁻⁸mATP in 1% yeast extract solution) the treatment with adenosine phosphate deaminase resulted in the reduction of ATP to 1.3 × 10⁻¹¹m, and the concomitant use of apyrase lowered the concentration to 3.3 × 10⁻¹³m. The treatment (0.05 U/ml of adenosine phosphate deaminase and apyrase) was applied to the detection of bacteria in broth by the L-L method, affording the detection of 42 colony-forming unit (CFU)/ml ofEscherichia coliand 10 CFU/ml ofStaphylococcus aureusin the broth.