Mitogenic and adjuvant activities of polysaccharides from the cellular slime mold,Dictyostelium discoideum NC-4

Cell surface and extracellular polysaccharide fractions obtained from Dictyostelium discoideum NC-4 cultured in bacteria-free medium showed strong B-cell mitogenic activities. Upon periodate treatment of the extracellular polysaccharide fraction this activity completely disappeared. The extracellular polysaccharide fraction could also enhance the antibody response in vitro against sheep red blood cells.     

A B Lymphocyte Mitogen Extracted from a Fungus Peziza vesiculosa1

A water-soluble mitogen was extracted with hot-water from the fruiting bodies of a fungus, Peziza vesiculosa, collected in the wild. The active substance, named vesiculogen, was able to stimulate selectively murine B cells because mitogenic activity was observed in the spleen cell cultures of congenitally athymic nude mice, but not in the thymus cell cultures. The possibility that the mitogenicity of vesiculogen was due to lipopolysaccharide was denied completely by the following evidence: 1) lipopolysaccharide in vesiculogen was undetectable (less than 0.001% in the Limulus test), 2) vesiculogen was able to stimulate strongly DNA synthesis of spleen cells from C3H/HeJ mice, and 3) the mitogenic activity of vesiculogen was not inhibited by polymyxin B. Vesiculogen increased antigen-nonspecifically the number of direct plaque forming cells to sheep erythrocytes, horse erythrocytes, and trinitrophenylated-horse erythrocytes. This result shows that vesiculogen acts as a polyclonal B cell activator on murine spleen cells.     

Campestroside,a new tetrahydroxanthone glucoside from Gentiana campestris

Campestroside has been isolated from the aerial parts of Gentiana campestris. From UV, MS, ¹H-NMR and ¹³C-NMR data its structure has been established as 1,3,5-trihydroxy-8-β-d-glucopyranosyl-5,6,7,8-tetrahydroxanthone. Campestroside which has also been detected in G. ramosa and G. germanica is the first reported tetrahydroxanthone glycoside.     

Construction of a supF-based system for detection of mutations in the chromosomal DNA of Arabidopsis

The factors maintaining genomic integrity, which have been studied in detail in other species, have yet to be investigated in plants. Recent progress in gene-silencing technology has made it possible to produce transgenic plants with loss-of-function phenotypes for the effective analysis of these factors, even with the high redundancy of genes in plants. Therefore, a mutation-detection system for plants is necessary to estimate the biological function of a target gene for mutation frequencies and spectra. Here, we reported the development of a novel system to analyze mutations in the chromosomal DNA of plants. The supF gene of E. coli was used as a target for the mutation because it was possible to detect all mutational base changes. Based on the plasmid pTN30, which carries supF, we constructed a binary Ti vector for its introduction to Arabidopsis genomes. The system was validated by measuring mutations in both non-treated and mutagen-treated transgenic plants. DNA fragments including pTN30 were rescued from the plants, and introduced into E. coli KS40/pOF105 to isolate the supF mutant clones conferring both nalidixic acid and streptomycin resistance on transformants. We found that the mutation frequency was approximately three times higher with the ethyl methanesulfonate (EMS) treatment than without it and G:C to A:T transitions dominated, which was the most reasonable mutation induced by EMS. These results show that this system allowed for the rapid analysis of mutations in plants, and may be useful for analyzing plant genes related to the functions of genomic stability and monitoring environmental genotoxic substances.     

Comparison of CGRP distributions in the maxillary sinus and trigeminal ganglion between elderly dentulous and edentulous humans

Thickening of the Schneiderian membrane (SM, mucosa of the maxillary sinus) appears in the paranasal sinus. Information on SM thickening is available for patients receiving sinus lift treatments, which is a risk factor for SM excretory dysfunction. However, more information is needed on the structure of the SM and the relationship between the maxilla sinus and palatine with the alveolar bone and the SM for dental implant treatment in the human maxilla. One hundred twenty-six sides of the maxilla from 71 cadavers were subjected to cone-beam computed tomography analysis and macroscopic and immunohistochemical observations in this study. A thickened SM was mainly observed in the middle region of the basal layer of the maxillary sinus (MS). Strong calcitonin gene-related peptide (CGRP)-positive reactions were observed in the alveolar bone, oral mucosa, mucosa of the MS, and trigeminal ganglion (TG) cells in dentulous samples compared with edentulous samples. TG cells play important roles in delivering CGRP through axons to the mucosal gland and in regulating the maxilla-related thickening of the SM. These data could help determine CGRP functions in the mucosal gland and bone formation between dentulous and edentulous samples and indicate that CGRP may pass from the TG to the MS glands.Key words: Mucosa, maxillary sinus, cone-beam computed tomography, immunohistochemistry, calcitonin gene-related peptide, trigeminal ganglion     

A rapid increase in lysophospholipids after geranylgeranoic acid treatment in human hepatoma-derived HuH-7 cells revealed by metabolomics analysis

Geranylgeranoic acid (GGA) was developed as a preventative agent against second primary hepatoma, and was reported to induce cell death in human hepatoma cells via Toll-like receptor 4 (TLR4)-mediated pyroptosis. We recently reported that GGA is enzymatically biosynthesized from mevalonic acid in human hepatoma-derived HuH-7 cells and that endogenous GGA is found in most rat organs including the liver. An unbiased metabolomics analysis of ice-cold 50% acetonitrile extracts from control and GGA-treated cells was performed in this study to characterize the intracellular metabolic changes in GGA-induced pyroptosis and to analyze their relationship with the mechanism of GGA-induced cell death. The total positive ion chromatograms of the cellular extracts in ultra-performance liquid chromatography coupled with quadrupole time-of-flight mass spectrometry were apparently unchanged after GGA treatment, but an orthogonal partial least squares-discriminant analysis score plot clearly discriminated the intracellular metabolite profiles of GGA-treated cells from that of control cells. S-plot analysis revealed 15 potential biomarkers up-regulated by 24-h GGA treatment according to their variable importance in the projection value of more than 1, and the subsequent metabolomics analysis identified nine of these metabolites as a group of lysophospholipids containing lysophosphatidylcholine with C16:0, C20:4, or C20:3 fatty acids. The possible roles of these lysophospholipids in GGA-induced pyroptosis are discussed.     

Two triterpenoid glycosides from leaves of Ilex cornuta

Two new triterpene glycosides, a diglycoside (as the corresponding methyl ester) and a bis-desmoside were isolated from leaves of Ilex cornuta. The     

Gene expression profiles of novel caprine placental prolactin-related proteins similar to bovine placental prolactin-related proteins

Background  

This study reports the identification of a full-length cDNA sequence for two novel caprine prolactin-related proteins (cPRP1 and cPRP6), and their localization and quantitative expression in the placenta. Caprine PRPs are compared with known bovine PRPs. We examined their evolution and role in the ruminant placenta.     

Inter- and intraspecific interactions among larvae of specialist and generalist parasitoids

Intra- and interspecific larval interactions that take place in a host body were investigated for two tachnid fliesEpicampocera succincta andCompsilura concinnata (Diptera: Tachinidae) parasitizingPieris butterfly larvae.E. succincta, a specialist onPieris butterflies, showed contest-type intraspecific competition, eliminating all the other conspecific larvae. On the other hand, an extreme generalist parasitoidC. concinnata exhibited scramble-type competition, sharing the host with other conspecifics and suffering reduced body size as a result. However, when these two species occurred together in a single host,C. concinnata had a much higher chance of survival. Moreover,C. concinnata could often survive in the presence of a parasitoid waspCotesia glomerata (Hymenoptera: Braconidae) whileE. succincta could not. The high tolerance ofC. concinnata could be attributable to its being an extreme generalist: To attack and survive on many different hosts, one has to be able to deal with various competitors. The competitive inferiority of the specialistE. succincta, on the other hand, may be a result of relatively recent encounter with, those competitors.     

Functional changes in troponin T by a splice donor site mutation that causes hypertrophic cardiomyopathy

A splice donorsite mutation in intron 15 of the cardiac troponin T (TnT) gene hasbeen shown to cause familial hypertrophic cardiomyopathy (HCM). In thisstudy, two truncated human cardiac TnTs expected to be produced by thismutation were expressed in Escherichiacoli and partially (50-55%) exchanged into rabbit permeabilized cardiac muscle fibers. The fibers into which a short truncated TnT, which lacked the COOH-terminal 21 amino acids because ofthe replacement of 28 amino acids with 7 novel residues, had beenexchanged generated aCa²⁺-activated maximum force thatwas slightly, but statistically significantly, lower than thatgenerated by fibers into which wild-type TnT had been exchanged whentroponin I (TnI) was phosphorylated by cAMP-dependent protein kinase. Along truncated TnT simply lacking the COOH-terminal 14 amino acids hadno significant effect on the maximum force-generating capability in thefibers with either phosphorylated or dephosphorylated TnI.Both these two truncated TnTs conferred a lower cooperativity and ahigher Ca²⁺ sensitivity on theCa²⁺-activated force generationthan did wild-type TnT, independent of the phosphorylation of TnI bycAMP-dependent protein kinase. The results demonstrate that the splicedonor site mutation in the cardiac TnT gene impairs the regulatoryfunction of the TnT molecule, leading to an increase in theCa²⁺ sensitivity, and a decreasein the cooperativity, of cardiac muscle contraction, which might beinvolved in the pathogenesis of HCM.