Characterization of immunoreactive endothelin in human urine.

We developed three antibodies, specific and sensitive to endothelin-1 (ET-1), and established two sandwich and three competitive enzyme immunoassays (EIAs). By using these EIAs, large immunoreactive ET (IR-ET) of molecular weight 10 k Da was identified as a main component of IR-ETs in human urine. This large IR-ET, which reacted with two antibodies specific for N-terminal region of ET-1 but not with the antibody against C-terminal peptide of ET-1, was partially purified by six-step procedure and examined by Western blotting after SDS polyacrylamide gel electrophoresis. The large IR-ET was detected as a single band at molecular weight of 10 k Da both in reduced and non-reduced conditions. From these results, the large IR-ET was thought to consist of a single polypeptide chain and possess the steric restricted N-terminal region of ET-1.     

Regional distribution of prostaglandin endoperoxide synthase studied by enzyme-linked immunoassay using monoclonal antibodies

Prostaglandin endoperoxide synthase transforms arachidonic acid to prostaglandin H2 via prostaglandin G2. The enzyme purified from bovine vesicular gland was given to mice as antigen, and monoclonal antibodies were raised by the hybridoma technique. Two species of the monoclonal antibody recognizing different sites of the enzyme were utilized to establish a peroxidase-linked immunoassay of prostaglandin endoperoxide synthase. Fab' fragment of one of the antibodies was prepared and conjugated to horseradish peroxidase. The conjugate was then bound to prostaglandin endoperoxide synthase, and the labeled enzyme was precipitated by the addition of the other antibody. The peroxidase activity of the immunoprecipitate correlated linearly with the amount of prostaglandin endoperoxide synthase. This sensitive and convenient method to determine the enzyme amount rather than the enzyme activity was utilized to extensively screen the amount of prostaglandin endoperoxide synthase in various bovine tissues. In addition to vesicular gland, platelets and kidney medulla previously known as rich enzyme sources, the immunoenzymometric assay demonstrated a high content of the enzyme in various parts of alimentary tract and a low but significant amount of enzyme in some parts of brain.     

Sago Palm (Metroxylon Sagu, Arecaceae) production in the Eastern Archipelago of Indonesia: Variation in morphological characteristics and pith dry-matter yield

Eleven local varieties of sago palm (Metroxylon sagu Rottb.) in southeast and north Sulawesi and in northern Maluku were studied: one variety with a weak black band on the back of the petiole: three varieties with a brown band on the back of the petiole: seven bandless varieties comprising two spineless, four short spine and one long spine types. Large variation in morphological characteristics and pith dry-matter yield were estimated at 13 to 34% and 55%, respectively. The difference in pith dry-matter yield is mainly attributed to trunk diameter and dry-matter percentage of pith. Trunk diameter was not affected by the length of growth period, which might reflect the palm’s own characteristics, such as genetic background and growth environment. The dry-matter percentage of pith was not related to any characteristics measured. The pith dry-matter yield was highest in the short spine type, followed by the spineless and the long spine types.

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Produksi Palma Sagu (Metroxylon Sagu, Arecaceae) Di Kepulauan Timur Indonesia: Keragaman Karakteristik Morfologi Dan Hasil Bahan Kering Empulur Batang

Résumé  Dalam survey tersebut dipelajari sebelas varitas sagu lokal (Metroxylon sagu Rottb.) di Sulawesi Tenggara, Sulawesi Utara, dan Maluku Utara: satu varitas dengan pita sedikit hitam pada bagian belakang dari tulang daun: tiga varitas dengan pita coklat pada bagian belakang belakang dari tulang daun: tujuh varitas tanpa pita terdiri dari dua varitas tanpa duri, empat varitas duri pendek dan satu varitas duri panjang. Terdapat adanya keragaman pada karakteristik morfologi dan hasil bahan kering empulur batang yang diperkirakan beriurut-turut berkisar 13 sampai 34% dan 55%. Perbedaan pada hasil bahan kering empulur batang terutama tergantung pada diameter batang dan proporsi kering empulur batang. Diameter batang tidak dipengaruhi oleh panjangnya periode tumbuh; namun nampaknya lebih terkait dengan gambaran karakteristik khusus, seperti latar belakang genetik dan lingkungan tumbuhnya.Persen bobot kering empulur batang tidak ada hubungannya dengan berbagai karakteristik yang diteliti. Hasil bahan kering empulur batang tertinggi adalah pada tipe duri pendek (511kg/batang), diikuti tipe tanpa duri (417kg/batang) dan tipe duri panjang (329kg/batang).

     

Relationship between localization on cellular membranes and cytotoxicity of Vibrio vulnificus hemolysin

Vibrio vulnificus secretes a hemolysin/cytolysin (VVH) that induces cytolysis in target cells. A detergent resistant membrane domain (DRM) fraction of the cells after sucrose gradient centrifugation includes cholesterol-rich membrane microdomains which have been called "lipid rafts". It was reported that some pore-forming toxins require association with DRM and/or lipid rafts to exert their cytotoxicity. It has also been thought that cellular cholesterol is involved in VVH cytotoxicity because VVH cytotoxicity was inhibited by pre-incubation with cholesterol. However, both cellular localization and mode of action of VVH cytotoxicity remain unclear. In this study, we investigated the relationship between VVH localization on the cellular membrane and its cytotoxicity. Oligomers of VVH were detected from DRM fractions by sucrose gradient ultracentrifugation but all of these oligomers shifted from DRM fractions to non-DRM fractions after treatment with methyl-beta-cyclodextrin (MβCD), a cholesterol sequestering agent. On the other hand, immunofluorescence analysis showed that VVH did not co-localize with major lipid raft markers on cellular membrane of CHO cells. These data suggested that VVH localized at membrane regions which are relatively abundant in cholesterol but which are not identical with lipid rafts. To determine the linkage between localization and cytotoxicity of VVH, cytotoxicity was evaluated in MβCD-treated CHO cells. The cytotoxicity of VVH was not decreased by the MβCD treatment. In addition, the amount of VVH oligomer did not decrease in MβCD-treated CHO cells. Thus, we found that the amount of oligomer on cellular membrane is important for induction of cytotoxicity, whereas localization to lipid rafts on the cellular membrane was not essential to cytotoxicity.     

Directionally Evolving Genetic Code: The UGA Codon from Stop to Tryptophan in Mitochondria

For the comprehensive analyses of deviant codes in protistan mitochondria (mt), we sequenced about a 1.1-kb region of a mitochondrial (mt) gene, the cytochrome c oxidase subunit I (coxI) in two chlorarachniophytes, the filose amoeba Euglypha rotunda, the cryptomonad Cryptomonas ovata, the prymnesiophyte (haptophyte) Diacronema vlkianum (Pavlovales), and the diatom Melosira ambigua. As a result of this analysis, we noticed that the UGA codon is assigned to tryptophan (Trp) instead of being a signal for translational termination in two chlorarachniophytes and in E. rotunda. The same type of deviant code was reported previously in animals, fungi, ciliates, kinetoplastids, Chondrus crispus (a red alga), Acanthamoeba castellanii (an amoeboid protozoon), and three of the four prymnesiophyte orders with the exception of the Pavlovales. A phylogenetic analysis based on the COXI sequences of 56 eukaryotes indicated that the organisms bearing the modified code, UGA for Trp, are not monophyletic. Based on these studies, we propose that the ancestral mitochondrion was bearing the universal genetic code and subsequently reassigned the codon to Trp independently, at least in the lineage of ciliates, kinetoplastids, rhodophytes, prymnesiophytes, and fungi. We also discuss how this codon was directionally captured by Trp tRNA. Received: 26 January 1998 / Accepted: 24 April 1998     

The Aromatic Ring of Phenylalanine 334 Is Essential for Oligomerization of Vibrio vulnificus Hemolysin

Vibrio vulnificus hemolysin (VVH) is thought to be a member of the cholesterol-dependent cytolysin (CDC) family of pore-forming toxins. To date, the structure-function relationships of CDCs produced by Gram-negative bacteria remain largely unknown. We show here that the aromatic ring of phenylalanine residue conserved in Vibrionaceae hemolysins is essential for oligomerization of VVH. We generated the VVH mutants; substituted Phe 334 for Ile (F334I), Ala (F334A), Tyr (F334Y), or Trp (F334W); and tested their binding and oligomerizing activity on Chinese hamster ovary cells. Binding in all mutants fell by approximately 50% compared with that in the wild type. Oligomerizing activities were completely eliminated in F334I and F334A mutants, whereas this ability was partially retained in F334Y and F334W mutants. These findings indicate that both hydrophobicity and an aromatic ring residue at the 334th position were needed for full binding activity and that the oligomerizing activity of this toxin was dependent on the existence of an aromatic ring residue at the 334th position. Our findings might help further understanding of the structure-and-function relationships in Vibrionaceae hemolysins.Vibrio vulnificus hemolysin (VVH) is a pore-forming toxin produced by the Gram-negative bacterium Vibrio vulnificus (6, 11). VVH binds directly to cholesterol and is oligomerized in vitro. Once VVH forms the VVH-cholesterol complex, it can no longer bind to susceptible cells (10). Therefore, VVH could be considered a member of the cholesterol-dependent cytolysin (CDC) toxin family (35).A wide variety of Gram-positive and some Gram-negative bacteria produce CDCs, which require cellular cholesterol to exert their cytotoxicity (22, 38). Structure-function relationships between CDCs produced by Gram-positive bacteria (gpCDCs) have been studied intensively for over a decade, whereas CDCs produced by Gram-negative bacteria remain largely unknown. On the other hand, it is well known that some Vibrionaceae bacteria, such as Vibrio vulnificus, Vibrio cholerae, Aeromonas hydrophila, and Aeromonas sobria, produce pore-forming toxins/hemolysins. Among them, it was reported that VVH and Vibrio cholerae cytolysin (VCC) required cholesterol to exert their activity (12, 35). Thus, Vibrionaceae hemolysins are thought to be members of the CDC family. The generalized toxic steps are thought to be similar for both gpCDCs and Vibrionaceae hemolysins (22); i.e., monomers interact with a susceptible cell membrane, these monomers are assembled to form oligomers by membrane fluidity, and transmembrane pore formation follows (5, 22, 27, 30, 37). Although gpCDCs and Vibrionaceae hemolysins have common toxic steps, the following differences exist between them. (i) There is no similarity in amino acid sequences. (ii) gpCDCs have a highly conserved tryptophan-rich motif, which is involved in membrane recognition (3, 9, 27), whereas this motif does not exist in Vibrionaceae hemolysins. (iii) gpCDCs, such as perfringolysin and intermedilicine, are composed of four domains, whereas Vibrionaceae hemolysins are composed of two or three domains (21, 24, 25). (iv) Vibrionaceae hemolysins form pores that are smaller (2 to 3 nm in diameter) (33, 36) than those formed by gpCDCs (approximately 30 nm) (1, 2, 19).Recently, the crystal structure of VCC was determined (21). VCC is composed of three domains, namely the cytolysin domain, the β-trefoil lectin domain, and the β-prism lectin domain (21). The proposed mechanisms of action of VCC are as follows: (i) monomer binding to cell surfaces via interactions with the cytolysin domain, (ii) binding to carbohydrate receptors by the β-prism lectin domain, (iii) oligomerization via the cytolysin domain, and (iv) pore formation by insertion of a stem-loop from the cytolysin domain into the cellular membrane (21). On the other hand, from the analysis of the VVH amino acid sequence, it has been predicted that VVH is composed of two domains (21) and is missing the β-prism lectin domain, which binds to carbohydrate receptors on the cellular membrane (21). Therefore, the structure and functions of VVH are thought to be slightly different from those of VCC. Thus, analysis of the structure-function relationship of VVH will aid in the understanding of the evolutionary process of CDCs as well as of the toxic mechanism of VVH.In this study, we show that phenylalanine in the 334th position (F334) is required for the binding and oligomerizing ability of VVH. In particular, the benzene ring of this phenylalanine is a prerequisite for its oligomerizing ability. Because of the high conservation of this phenylalanine in other Vibrionaceae hemolysins, our results will contribute to a better understanding of the structure-function relationships of Vibrionaceae hemolysins.     

Increased Expression of DNA Methyltransferase 3a in Obese Adipose Tissue: Studies With Transgenic Mice

Epigenetic mechanisms are likely to be involved in the development of obesity. This study was designed to examine the role of a DNA methyltransferase (Dnmt3a), in obese adipose tissue. The gene expression of Dnmts was examined by quantitative real‐time PCR analysis. Transgenic mice overexpressing Dnmt3a in the adipose tissue driven by the aP2 promoter were created (Dnmt3a mice). DNA methylation of downregulated genes was examined using bisulfite DNA methylation analysis. Dnmt3a mice were fed a methyl‐supplemented or high‐fat diet, and subjected to body weight measurement and gene expression analysis of the adipose tissue. Expression of Dnmt3a was markedly upregulated in the adipose tissue of obese mice. The complementary DNA (cDNA) microarray analysis of Dnmt3a mice revealed a slight decrease in the gene expression of secreted frizzled‐related protein 1 (SFRP1) and marked increase in that of interferon responsive factor 9 (IRF9). In the SFRP1 promoter, DNA methylation was not markedly increased in Dnmt3a mice relative to wild‐type mice. In experiments with a high‐fat diet or methyl‐supplemented diet, body weight did not differ significantly with the genotypes. Gene expression levels of inflammatory cytokines such as tumor necrosis factor‐α (TNF‐α) and monocyte chemoattractant protein‐1 (MCP‐1) were higher in Dnmt3a mice than in wild‐type mice on a high‐fat diet. This study suggests that increased expression of Dnmt3a in the adipose tissue may contribute to obesity‐related inflammation. The data highlight the potential role of Dnmt3a in the adult tissue as well as in the developing embryo and cancer.     

Distribution of the pulmonary artery and vein in the lung of the white handed gibbon

The lungs of four white handed gibbons (Hylobates agilis) were examined. The right pulmonary artery runs across the ventral side of the right upper lobe bronchiole, and then traverses the dorsal side of the right middle lobe bronchiole. Thereafter, it runs along the dorso-lateral side of the right bronchus, between the dorsal bronchiole system and the lateral bronchiole system, and gradually follows the dorsal side of the right bronchus. During its course, it gives off arterial branches which run along each bronchiole. The left pulmonary artery runs across the dorsal side of the left middle lobe bronchiole and then along the left bronchus as in the right lung. The branches of the pulmonary artery run mainly along the dorsal or lateral side of the bronchiole, while the pulmonary veins run mainly the medial side of the bronchioles or between them. However, in a few portions, the pulmonary veins run the lateral side of the bronchioles. Finally, they enter the left atrium with four large veins i.e. the common trunk of the right upper lobe vein and right middle lobe vein, right lower lobe pulmonary venous trunk, left middle lobe vein, and left lower lobe pulmonary venous trunk.