[The C-MAC videolaryngoscope: its utility in tracheal intubation by novice personnel].

Background: The aim of this study was to evaluate the suitability of the C-MAC videolaryngoscope for the tracheal intubation especially by novice personnel.

Methods: Endotracheal intubation was performed using the C-MAC videolaryngoscope in 40 patients undergoing general anesthesia. We compared the percentage of glottic opening score between Macintosh laryngoscope and the C-MAC videolaryngoscope by anesthesia staff and novice personnel.

Experimental and theoretical aspects of the haptotropic rearrangement of diiron and diruthenium carbonyl complexes bound to 4,6,8-trimethylazulene.

The haptotropic rearrangement of dinuclear metal carbonyl species on the conjugate pi-ligand of (micro2,eta3:eta5-4,6,8-trimethylazulene)M2(CO)5 [M = Fe (3) and Ru (4)] was investigated in detail both experimentally and theoretically. The complexes, 3 and 4, were synthesized and characterized by spectroscopy and crystallography. The spin saturation transfer technique of 1H NMR was used to measure the rate constant k of the haptotropic isomerization between the two enantiomers of 3 and 4, from which thermodynamic parameters were determined: (3; deltaS(double dagger) = -7 +/- 1 cal K(-1) mol(-1), deltaH(double dagger) = 22 +/- 1 cal mol(-1), deltaG(double dagger)373 = 25 +/- 1 cal mol(-1)), (4; deltaS(double dagger) = 7 +/- 1 cal K(-1) mol(-1), deltaH(double dagger) = 25 +/- 1 cal mol(-1), deltaG(double dagger)373 = 23 +/- 1 cal mol(-1)).

Developmentally-regulated expression of tissue-specific splice variant of rat vesicular glutamate transporter 1 in retina and pineal gland.

Three distinct subtypes of vesicular glutamate transporters (VGLUTs) have been identified to date that are expressed basically in a cell type-specific manner. We have found a splice variant of VGLUT1 mRNA that is expressed almost exclusively in photosensitive tissues, i.e.

Usefulness of deoxyribonuclease I (DNase I) polymorphism for individualization from small aged urine stains.

We devised a procedure that combines a simple extraction method, isoelectric focusing and activity staining using the dried agarose film overlay method, for deoxyribonuclease I (DNase I) typing from aged urine stains. DNase I types were determined without difficulty from urine stains kept at room temperature for 3 months or more in all of the samples tested. The amounts of urine stains required for typing after 3 months of storage were estimated to be equivalent to 60-120 microl of liquid urine.

Expression of inorganic phosphate/vesicular glutamate transporters (BNPI/VGLUT1 and DNPI/VGLUT2) in the cerebellum and precerebellar nuclei of the rat.

Expression of inorganic phosphate/vesicular glutamate transporters (BNPI/VGLUT1 and DNPI/VGLUT2) was studied in the cerebellum and precerebellar nuclei of rats using immunohistochemistry and in situ hybridization. DNPI/VGLUT2-stained mossy fibers were principally seen in the vermis (lobules I and VIII-X) and flocculus, whereas BNPI/VGLUT1-stained mossy fibers were localized throughout the cortex. Some vermal and floccular mossy fibers were stained for both transporters.

Differential expression of two distinct vesicular glutamate transporters in the rat retina.

Expression and cellular localization of vesicular glutamate transporters (BNPI and DNPI) were studied in the rat retina. RT-PCR showed expression of both transporter mRNAs. hybridization demonstrated BNPI mRNA signals in the inner segments of photoreceptors and the inner nuclear layer, whereas DNPI mRNA signals were confined to the ganglion cell layer.

A composite hormone response element regulates transcription of the rat GHRH receptor gene.

To further elucidate the molecular mechanisms underlying the transcriptional regulation of the GHRH receptor (GHRH-R) gene, hormonal regulation of the promoter activity of this gene was examined. An approximately 3-kb genomic fragment spanning the promoter region of the gene was sequenced and the transcription start site was determined by RT-PCR and RNase protection assay. A major start site was localized at -105 (relative to the translation initiation codon, ATG), and a pit-1 binding sequence characteristic of pituitary specific genes was found at -155 to -146.