Livre des Morts de Nésyménou. Egyptien 123

Fragment 3 :Col. 1 + vignette (très fragmentaires) : ?Col. 2 + vignette : chapitre 86 (formule pour prendre l'aspect d'une hirondelle). La vignette contient une hirondelle sur une butte.Col. 3 + vignette : chapitre 87 (formule pour prendre l'aspect d'un serpent-sata). La vignette montre un serpent à tête humaine. Col. 4 + vignette : chapitre 88 (formule pour faire une transformation en crocodile Sobek). La vignette montre une crocodile momiforme.Col. 5 + vignette : chapitre 89 (formule pour permettre que la ba atteigne son cadavre dans la nécropole). La vignette montre l'oiseau-ba volant au-dessus du cadavre allongé sur le lit funéraire.Col. 6 + vignette (fragmentaires) : chapitre 90 (?). La vignette montre le défunt debout les bras en avant.Fragment 2 :Col. 1 + vignette (fragmentaires) : ? Seul un morceau de la vignette est conservé où l'on voit une divinité debout.Col. 2 + vignette : chapitre 91 (formule pour ne pas retenir le ba du défunt dans la nécropole). La vignette montre le défunt debout devant son oiseau-ba.Col. 3 + vignette : chapitre 92 (formule pour ouvrir la tombe pour le ba et pour l'ombre du défunt pour sa sortie pendant le jour). La vignette représente le défunt devant une chapelle où l'on voit l'oiseau-ba.Col. 4 + vignette : chapitre 93 (formule pour ne pas permettre que le défunt ne traverse vers l'Orient dans la nécropole). La vignette représente une divinité assise sur une barque avec le signe de l'Orient.Col. 5 + vignette (voir cadre suivant) : début du chapitre 98 (formule pour aller chercher le bac dans le ciel). La vignette montre la proue de la barque.Fragment 1 (prend place au sein des fragments du cadre suivant Egyptien 122) :Col. 1 + vignette : chapitre 102 (formule pour descendre dans la barque). La vignette représente Rê assis sur sa barque.Col. 2 + vignette (fragmentaires) : ? La vignette laisse deviner une barque.

Molecular cytogenetic analysis of heterochromatin in the chromosomes of tilapia, Oreochromis niloticus (Teleostei : Cichlidae)

The structure of the heterochromatic bands in mitotic chromosomes of the important tropical aquaculture species of tilapia, Oreochromis niloticus, was investigated by the combination of the C-banding technique, chromosomal digestion with two restriction endonucleases and fluorescence in situ hybridization (FISH) of two satellite DNAs (SATA and SATB). The tilapia chromosomes presented heterochromatic bands in the centromeres and in the short arms of almost all chromosomes that were differentially digested by the restriction endonucleases HaeIII and EcoRI. FISH of SATA showed that the satellite sequence is distributed in the centromeric region of all chromosomes of tilapia. FISH also revealed an intense hybridization signal for SATB in only one chromosome pair, but less intense signals were also present in several other pairs. The digestion of tilapia chromosomes by HaeIII and EcoRI was positively correlated with the position of SATA and SATB in chromosomes as revealed by FISH. The results obtained may be useful in future molecular and genetic studies of tilapias.

Chromosome Evolution in African Cichlid Fish: Contributions from the Physical Mapping of Repeated DNAs

Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)

Characterisation of the chromosome fusions in Oreochromis karongae

Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)

The B chromosomes of the African cichlid fish Haplochromis obliquidens harbour 18S rRNA gene copies

Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)

Effects of phonophoresis with Arnica montana onto acute inflammatory process in rat skeletal muscles: An experimental study

This study aimed at verifying the effects of phonophoresis associated with Arnica montana on the acute phase of an inflammatory muscle lesion. Forty Wistar male rats (300 +/- 50 g), of which the Tibialis Anterior muscle was surgically lesioned, were divided into four groups (n = 10 each): control group received no treatment; the ultrasound group (US) was treated in pulsed mode with 1-MHz frequency, 0.5 W/cm(2) intensity (spatial and temporal average - SATA), duty cycle of 1: 2 (2 ms on, 4 ms off, 50%), time of application 3 min per session, one session per day, for 3 days; the phonophoresis or ultrasound plus arnica (US+A) group was treated with arnica with the same US parameters plus arnica gel; and the arnica group (A) was submitted to massage with arnica gel, also for 3 min, once a day, for 3 days. Treatment started 24 h after the surgical lesion. on the 4th day after lesion creation, animals were sacrificed and sections of the lesioned, inflamed muscle were removed for quantitative (mononuclear and polymorphonuclear cell count) and qualitative histological analysis. Collected data from the 4 groups were statistically analyzed and the significance level set at p < 0.05. Results show higher mononuclear cell density in all three treated groups with no significant difference between them, but values were significantly different (p < 0.0001) when compared to control group's. As to polymorphonuclear cell density, significant differences were found between control group (p = 0.0134) and US, US+A and A groups; the arnica group presented lesser density of polymorphonuclear cells when compared (p = 0.0134) to the other groups. No significant difference was found between US and US+A groups. While the massage with arnica gel proved to be an effective anti-inflammatory on acute muscle lesion in topic use, these results point to ineffectiveness of Arnica montana phonophoresis, US having seemingly checked or minimized its anti-inflammatory effect. (C) 2008 Elsevier B. V. All rights reserved.

Calibration of therapeutic ultrasound equipment

Temporal and spatial acoustic intensity (SATA) of therapeutic ultrasound (US) equipment should be monitored periodically. In order to evaluate the conditions of US equipment in use in the city of Piracicaba-Sao Paulo, Brazil, 31 machines - representing all Brazilian manufacturers - were analysed under continuous and pulsed conditions at a frequency of 1 MHz. Data about temporal and spatial acoustic intensity were collected and the use of equipment was surveyed. Intensities of 0.1, 0.2, 0.5, 0.8, 1.0, 1.5, 2.0, 2.5 and 3.0 Wcm -2, indicated on the equipment panel were analysed using a previously calibrated digital radiation pressure scale, model UPM-DT-1 (Ohmic Instruments Co). The acoustic intensity (I) results were expressed as superior and inferior quartile ranges for transducers with metal surfaces of 9 cm 2 and an effective radiation area (ERA) Of 4 cm 2. The results under continuous conditions were: I 0.1 = -20.0% and -96%. I 0.2 = -3.1% and -83.7%. I 0.5 = -35.0% and -86.5%. I 0.8 = -37.5% and -71.0%. I 2.5 = -49.0% and -69.5%. I 3.0 = -58.1% and -77.6%. For pulsed conditions, intensities were: I 0.1 = -40.0% and -86.2%. I 1.0 = -50.0% and -86.5%. I 1.5 = -62.5% and -82.5%. I 2.0 = -62.5% and -81.6%. I 2.5 = -64.7% and -88.8%. I 3.0 = -87.1% and -94.8%. In reply to the questionnaire drawn up to check the conditions of use of equipment, all users reported the use of hydrosoluble gel as a coupling medium and none had carried out previous calibrations. Most users used intensities in the range of 0.4. to 1.0 Wcm -2 and used machines for 300 to 400 minutes per week. The majority of machines had been bought during the previous seven years and weekly use ranged from less than 100 minutes to 700 minutes (11 hours 40 minutes). Findings confirm previous observations of discrepancy between the intensity indicated on the equipment panel and that emitted by the transducer and highlight the necessity for periodic evaluations of US equipment.

Citogenética comparativa de peixes da família Cichlidae

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES)

Mapeamento cromossômico comparativo em peixes ciclícos utilizando sequências repetitivas de DNA

Coordenação de Aperfeiçoamento de Pessoal de Nível Superior (CAPES)

Comparação do ultrassom pulsado e contínuo no reparo tendíneo de ratos

No tratamento de lesões tendíneas, o uso do ultrassom surge como possibilidade terapêutica, apesar de lacunas sobre seus efeitos clínicos. O objetivo foi avaliar dois protocolos de ultrassom terapêutico sobre dor e edema após trauma tendíneo. Vinte e um ratos Wistar foram submetidos a trauma no tendão calcâneo e divididos em três grupos: sham (GS); ultrassom contínuo (GUC); e ultrassom pulsado (GUP). O trauma ocorreu sobre a face lateral do tendão calcâneo direito, com energia de 0,40 J. A dor foi avaliada pelo teste de incapacidade funcional e o edema, pelo diâmetro laterolateral. Foram realizadas avaliações previamente à lesão; após 1 hora da indução da lesão; após o 1º tratamento; 2, 8 e 24 horas após lesão; e após o 5º dia. O tratamento ocorreu em 5 dias, com transdutor de 1 MHz, durante 3 minutos, sobre o local do trauma, com dose de 0,4 W/cm² SATA. Os resultados da incapacidade funcional para GS mostraram aumento da nocicepção. Para GUC houve aumento ao comparar a avaliação 1 (AV1) com as avaliações 2 (AV2), 3 (AV3) e 4 (AV4); ao comparar AV2 com as avaliações 5 (AV5) e 6 (AV6) houve diminuição de valores. Para GUP houve aumento ao comparar AV1 com AV2 e AV3, mas ao comparar AV2 com as seguintes, houve diminuição significativa a partir de AV4. Para o edema, os grupos tratados produziram aumento inicial, com redução nas últimas avaliações. O ultrassom terapêutico produziu diminuição de dor e edema, mais precocemente para a forma pulsada.

Nicht geträgerte Radioarsenisotope: ihre Herstellung, Abtrennung und Markierung von Proteinen

Das Element Arsen besitzt eine Reihe von Isotopen, die in nahezu trägerfreier Form (nca) produziert werden können und deshalb in der Radiopharmazie für die Diagnose oder Endoradiotherapie Verwendung finden können. Bei der Positronenemissionstomographie (PET) gibt es eine gewisse Lücke bei der Versorgung mit langlebigen Positronenemittern, die zur Untersuchung von langsamen physiologischen Prozessen wie z.B. der Biodistribution und Anreicherung von Antikörpern in Tumorgewebe eingesetzt werden können. Die beiden Arsenisotope 72As (T1/2 = 26 h, 88 % beta+) und 74As (T1/2 = 17,8 d, 29 % beta+) vereinen eine lange physikalische Halbwertszeit mit einer hohen Positronenemissionsrate und sind daher geeignete Kandidaten. Da das Verhalten von radioaktivem Arsen und seine Verwendung in der molekularen Bildgebung international relativ wenig bearbeitet sind, wurde die Radiochemie des Arsens von der Isotopenproduktion an Kernreaktor und Zyklotron, über die Entwicklung von Abtrennungsmethoden für Germanium und Arsen, bis hin zur Entwicklung einer soliden Markierungschemie für Antikörper weiterentwickelt. Die in dieser Arbeit bearbeiteten Felder sind: 1. Die Isotopenproduktion der relevanten Arsenisotope (72/74/77As) wurde an Kernreaktor und Zyklotron durch Bestrahlung von GeO2- und Germaniummetalltargets durchgeführt. Pro 6 h Bestrahlung von 100 mg Germanium konnten ca. 2 MBq 77As am TRIGA Reaktor in Mainz hergestellt werden. Am Zyklotron des DKFZ in Heidelberg konnten unter optimierten Bedingungen bei der Bestrahlung von Germaniummetall (EP = 15 Mev, 20 µA, 200 µAh) ca. 4 GBq 72As und ca. 400 MBq 74As produziert werden. 2. Die Entwicklung neuer Abtrennungsmethoden für nca 72/74/77As von makroskopischen Mengen Germanium wurde vorangetrieben. Für die Aufarbeitung von GeO2- und Germaniummetalltargets kamen insgesamt 8 verschiedene Methoden wie Festphasenextraktion, Flüssig-Flüssig-Extraktion, Destillation, Anionenaustauschchromatographie zum Einsatz. Die erzielten Ausbeuten lagen dabei zwischen 31 und 56 %. Es wurden Abtrennungsfaktoren des Germaniums zwischen 1000 und 1•10E6 erreicht. Alle erfolgreichen Abtrennungsmethoden lieferten *As(III) in 500 µl PBS-Puffer bei pH 7. Diese Form des Radioarsens ist für die Markierung von SH-modifizierten Molekülen, wie z.B. Antikörpern geeignet. 3. Die Entwicklung von Methoden zur Bestimmung des Oxidationszustandes von nca *As in organischem, neutralem wässrigen, oder stark sauren Medium mittels Radio-DC und Anionenaustauschchromatographie wurde durchgeführt und führte zu einem besseren Verständnis der Redoxchemie des nca *As. 4. SH-modifizierte Antikörper wurden mit 72/74/77As(III) markiert. Dabei wurden zwei Methoden (Modifizierung mit SATA und TCEP) miteinander verglichen. Während das *As(III) bei Verwendung von TCEP in Ausbeuten > 90 % mit dem Antikörper reagierte, wurde für SATA-modifizierte Antikörper in Abhängigkeit von der verwendeten Abtrennungsmethode eine breite Spanne von 0 % bis > 90 % beobachtet. 5. Es wurden Phantommessungen mit 18F, 72As und 74As am µ-PET-Scanner durchgeführt, um erste Aussagen über die zu erwartende Auflösung der Arsenisotope zu erhalten. Die Auflösung von 74As ist mit 18F vergleichbar, während die von 72As erkennbar schlechter ist.

Abundance and habitat covariates of lesser florican and spiny-tailed lizard in Kachchh, India (2008-09)

please provide abstract

Brefeldin A-inhibited guanine nucleotide-exchange activity of Sec7 domain from yeast Sec7 with yeast and mammalian ADP ribosylation factors

The Saccharomyces cerevisiae Sec7 protein (ySec7p), which is an important component of the yeast secretory pathway, contains a sequence of ≈200 amino acids referred to as a Sec7 domain. Similar Sec7 domain sequences have been recognized in several guanine nucleotide-exchange proteins (GEPs) for ADP ribosylation factors (ARFs). ARFs are ≈20-kDa GTPases that regulate intracellular vesicular membrane trafficking and activate phospholipase D. GEPs activate ARFs by catalyzing the replacement of bound GDP with GTP. We, therefore, undertook to determine whether a Sec7 domain itself could catalyze nucleotide exchange on ARF and found that it exhibited brefeldin A (BFA)-inhibitable ARF GEP activity. BFA is known to inhibit ARF GEP activity in Golgi membranes, thereby causing reversible apparent dissolution of the Golgi complex in many cells. The His6-tagged Sec7 domain from ySec7p (rySec7d) synthesized in Escherichia coli enhanced binding of guanosine 5′-[γ-[35S]thio]triphosphate by recombinant yeast ARF1 (ryARF1) and ryARF2 but not by ryARF3. The effects of rySec7d on ryARF2 were inhibited by BFA in a concentration-dependent manner but not by inactive analogues of BFA (B-17, B-27, and B-36). rySec7d also promoted BFA-sensitive guanosine 5′-[γ-thio]triphosphate binding by nonmyristoylated recombinant human ARF1 (rhARF1), rhARF5, and rhARF6, although the effect on rhARF6 was very small. These results are consistent with the conclusion that the yeast Sec7 domain itself contains the elements necessary for ARF GEP activity and its inhibition by BFA.

ARF-GEP100, a guanine nucleotide-exchange protein for ADP-ribosylation factor 6

A human cDNA encoding an 841-aa guanine nucleotide-exchange protein (GEP) for ADP-ribosylation factors (ARFs), named ARF-GEP100, which contains a Sec7 domain, a pleckstrin homology (PH)-like domain, and an incomplete IQ-motif, was identified. On Northern blot analysis of human tissues, a ≈8-kb mRNA that hybridized with an ARF-GEP100 cDNA was abundant in peripheral blood leukocytes, brain, and spleen. ARF-GEP100 accelerated [35S]GTPγS binding to ARF1 (class I) and ARF5 (class II) 2- to 3-fold, and to ARF6 (class III) ca. 12-fold. The ARF-GEP100 Sec7 domain contains Asp543 and Met555, corresponding to residues associated with sensitivity to the inhibitory effect of the fungal metabolite brefeldin A (BFA) in yeast Sec7, but also Phe535 and Ala536, associated with BFA-insensitivity. The PH-like domain differs greatly from those of other ARF GEPs in regions involved in phospholipid binding. Consistent with its structure, ARF-GEP100 activity was not affected by BFA or phospholipids. After subcellular fractionation of cultured T98G human glioblastoma cells, ARF6 was almost entirely in the crude membrane fraction, whereas ARF-GEP100, a 100-kDa protein detected with antipeptide antibodies, was cytosolic. On immunofluorescence microscopy, both proteins had a punctate pattern of distribution throughout the cells, with apparent colocalization only in peripheral areas. The coarse punctate distribution of EEA-1 in regions nearer the nucleus appeared to coincide with that of ARF-GEP100 in those areas. No similar coincidence of ARF-GEP100 with AP-1, AP-2, catenin, LAMP-1, or 58K was observed. The new human BFA-insensitive GEP may function with ARF6 in specific endocytic processes.

Human immunodeficiency virus type 1 reverse transcriptase: enhancement of activity by interaction with cellular topoisomerase I.

A number of studies have suggested that topoisomerase I (topo I) activity may be important in human immunodeficiency virus type 1 (HIV-1) replication. Specifically it has been reported that purified virus particles have topo I activity and that inhibitors of this enzyme can inhibit virus replication in vitro. We have investigated a possible association of HIV-1 gag proteins with topo I activity. We found that whereas the gag-encoded proteins by themselves do not have activity, the nucleocapsid protein p15 can interact with and enhance the activity of cellular topo I. Furthermore it could be demonstrated that topo I markedly enhanced HIV-1 reverse transcriptase activity in vitro and that this could be inhibited by the topo I-specific inhibitor camptothecin. The findings suggest that cellular topo I plays an important role in the reverse transcription of HIV-1 RNA and that the recruitment of this enzyme may be an important step in virus replication.