Molecular genetic study of interordinal relationships of mammals

Scally, M.

January 2002

No description available.

599

Mammalian evolution

Electrical and mechanical aspects of bladder contractility

Mostwin, J. L.

January 1986

No description available.

611

Mammalian bladder function

Comparative analyses of reproductive tactics

Read, Andrew F.

January 1989

No description available.

590

Mammalian reproductive cycles

Biochemical studies on biliary epithelial cells isolated from rat liver

Parola, Maurizio

January 1990

No description available.

572

Mammalian liver research

Analysis of dauer pathway genes in the parasitic nematode Trichinella spiralis

Boyd, Jacqueline

January 2003

<i>Trichinella spiralis</i> is a parasitic nematode of mammalian skeletal muscle.  Its life cycle includes two stages where developmental progression appears to be inhibited until a specific host niche is encountered.  The newborn larva, released within the host intestine depends upon entry to skeletal muscle for continued development.  The muscle larva encapsulates within skeletal muscle and further reproductive development is dependent upon ingestion by a new host.  Developmental arrest has been extensively characterised in <i>Caenorhabditis</i> <i>elegans</i>, where an alternative L3 larva, the dauer larva, is formed in response to environmental conditions refractive to continued reproductive development.  Using the wealth of genetic information regarding <i>C. elegans</i> dauer formation, putative periods of arrest were examined in <i>T. spiralis.</i> TGF-<span lang=EN-GB style='font-family:Symbol'>b-like and insulin-like signalling pathways are critical mediators of <i>C. elegans </i>dauer formation.  A <i>T. spiralis</i> TGF-<span lang=EN-GB style='font-family: Symbol'>b-ligand was identified and designated <i>ts-tll-1</i>.  Sequencing and analysis revealed <i>ts-tll-1</i> to be similar to vertebrate bone morphogenetic proteins and <i>C. elegans </i>DBL-1, is involved in body size regulation.  EST mining identified putative type I and II TGF-<span lang=EN-GB style='font-family:Symbol'>b receptors and a subtilsin-like proprotein convertase, suggesting conservation of TGF-<span lang=EN-GB style='font-family:Symbol'>b-like signalling in <i>T. spiralis.  </i>A partial <i>Trichinella </i>gene encoding an orthologue of the <i>C. elegans</i> insulin-like, tyrosine kinase receptor, DAF-2, was identified by degenerate PCR and designated <i>ts-tkr.  ts-tkr</i> is most similar to <i>C. elegans daf-2</i> within the highly conserved tyrosine kinase domain.  Two alternative transcripts of <i>ts-tkr</i> were identified by 3’ RACE, which differed in their 3’ UTRs.  Semi-quantitative RT-PCR analysis suggested <i>ts-tkr </i>expression was greatest in adult worms, implying a role in promoting reproductive development. Semi-quantitative RT-PCR was also to assess the expression of selected housekeeping and ES protein encoding genes during the <i>T. spiralis </i>life cycle.  While transcription in the <i>C. elegans</i> dauer is depressed, there was no obvious transcriptional repression in <i>Trichinella</i> newborn or muscle larva.

592.57

Mammalian skeletal muscle

The role of glycoconjugates in implantation

Hadad, Kameel

January 1990

No description available.

572

Mammalian fertilization

Characterisation of PSC1 as an acidic rich RS domain protein (ARRS) with a conserved mammalian family member.

Kavanagh, Steven James

January 2006

Title page, table of contents and summary only. The complete thesis in print form is available from the University of Adelaide Library. / The Acidic Rich family of RS Domain proteins (ARRS) is defined by both the presence and arrangement of conserved domains within 2 family members. Conserved regions include an RS domain, zinc finger domain, RNA binding motif and a C terminal acidic rich region. Two conserved motifs within the RRM of ARRS proteins have been defined that are not found in the RRM of other RNA binding proteins. Peri implantation stem cell 1 (pscl), the founding member of this family, was originally identified as a developmental marker differentially expressed between the Inner Cell Mass and primitive ectoderm of the mammalian embryo. Psc1 RNA is differentially up-regulated in the post gastrulation embryo and the adult, with high mRNA levels in lung, brain and kidney, and low level expression in other tissues. Comparative analysis of Psc1 to RS domain proteins known to function in mRNA processing, such as SC35 and ASF/SF2, has shown it colocalises to characteristic nuclear speckles. However, in contrast to SR proteins, Pscl localises to additional regions in the nucleus, not containing SR proteins, and to punctate regions in the cytoplasm termed cytospeckles. Further, in the absence of transcription, Psc 1 localises to regions in the nucleus which exclude nuclear speckles. Finally, unlike SC35 and ASF/SF2, which move rapidly in and out of nuclear speckles, FRAP assays show Psc1 is tethered within the nucleus. Analysis of Psc1 domain contribution to subcellular localisation and mobility shows the RRM to be both necessary and sufficient for Psc 1 cytospeckle localisation and is responsible for the nuclear tethering of Pscl. The RS domain of Pscl acts as a nuclear localisation signal and contributes to nuclear speckle localisation. The C terminal of Psc I localises with microtubules and is proposed to mediate Psc 1 cytoskeletal association. The expression of the Drosophila acidic rich RS domain protein (NP609976) is developmentally regulated in the same manner as Pscl, it has a nuclear localisation profile identical to Psc 1 and also localises to speckles in the cytoplasm, all of which support a conserved evolutionary role for Pscl and the ARRS protein family in mRNA processing and trafficking both in the nucleus and in the cytoplasm. / http://proxy.library.adelaide.edu.au/login?url= http://library.adelaide.edu.au/cgi-bin/Pwebrecon.cgi?BBID=1236604 / Thesis (Ph.D.) -- University of Adelaide, School of Molecular and Biomedical Science, 2006

acidic; protein; mammalian

Development of L1210 mutants in NAD metabolism

Sujareerat, Charin

January 1989

No description available.

572.8

Mammalian cell mutation

The role of PTHrP in murine placental development and function

Duval, Chloe

January 2014

Parathyroid hormone-related peptide (PTHrP) is abundantly expressed throughout the gestational tissues and has multiple roles in fetal development. The importance of PTHrP in embryonic growth and survival is emphasised by the retarded growth and peri-natal lethality of the PTHrP knockout mouse. PTHrP is a regulator of cell survival, proliferation and differentiation in a number of tissues and organs. However, its effects in the development and function of the placenta are yet to be fully defined. Therefore, the PTHrP knockout mouse was used to examine the morphological development and function of the placenta in the absence of fetal PTHrP gene expression. Embryos that were wild-type (WT), heterozygous (HZ) and null (NL) for the PTHrP allele were used for comparison. PTHrP expression was undetectable in the trophoblast cells of the NL placenta, with the HZ placenta exhibiting an intermediate phenotype. Placental development did occur in the absence of fetal PTHrP, although morphological abnormalities were apparent in the junctional zone and labyrinth zone at embryonic day (E)18. The NL placenta was frequently interrupted by large spaces and contained highly misshapen canals, which may reflect altered cellular and cell-matrix interactions. The area of the junctional zone on HZ and NL placental sections was reduced at E14 and E16, as was the area of the labyrinth zone of the NL placenta at E14 and E18. In culture, NL trophoblast cells had a lowered capacity for proliferation and survival. Elevated apoptosis was also observed in the HZ and NL placenta in vivo at E16 and E18, as judged by increased staining for the apoptotic marker, cleaved caspase-3. This effect was less pronounced in the HZ placenta. Evidence of increased insulin-like growth factor 2 (Igf2) expression was observed in the HZ and NL placenta at E14 and E16, which may have been a compensatory response to preserve some aspects of placental function in a PTHrP-deficient environment. Despite a reduced area of junctional and labyrinth zones on NL placental sections, no differences in placental weight was observed at any gestational age examined, which may indicate differences exist in the composition of the NL placenta. Fetal weight was lower in NL than WT fetuses at E16 and E18, whereas fetal weight in the HZ group was unaltered at these gestational ages. This suggests that the NL placenta had a more profoundly reduced capacity to support fetal growth. System A amino acid transport was significantly reduced in the NL placenta at E18, perhaps contributing to decreased NL fetal weight. Glycogen content of the NL placenta was reduced compared to WT at E12 and E14, but raised at E18, which may have been a compensatory mechanism to support fetal growth. In conclusion, PTHrP influences the morphological differentiation of the mouse placenta, trophoblast cell survival, nutrient transport and extraembryonic energy storage. PTHrP is an important regulator of placental development and function, which has associative effects on fetal growth and development.

612.6

Integrative Mammalian Biology

Serotonin in the blood of non-mammalian vertebrates

Simoneit, Lynda Wells

January 1965

Thesis (M.A.)--Boston University / PLEASE NOTE: Boston University Libraries did not receive an Authorization To Manage form for this thesis or dissertation. It is therefore not openly accessible, though it may be available by request. If you are the author or principal advisor of this work and would like to request open access for it, please contact us at open-help@bu.edu. Thank you. / The amount o serotonin, one of the biologically active amines, was determined in selected species of non-mammalian vertebrates - the dogfish Mustelus canis, the tautog Tautoga onitis, the turtle Pseudymys scripta elegans, and the chicken Gellus gallus. The extraction procedure employed was highly sensitive and specific. Contaminating indoles which occur naturally in tissues were removed before extraction by shaking with diethyl ether and adjusting the pH. Serotonin was then extracted with butanol from an alkaline, sodium chloride-saturated solution and re-extracted back into dilute acid. It was identified on a Farrand spectrophotofluorometer by its characteristic activation activation peak at 305 mu and fluorescence peak at 550 mu, and the amount present was determined. The range in chicken whole blood was found to be 10.3-19.4 ug. per ml. Under the conditions of the experiment, the major portion of chicken blood serotonin could not be shown to be contained in the thrombocytes. The range of serotonin in turtle whole blood was found to be .228-1.32 ug. per ml. Serotonin could not be demonstrated in the tautog or the dogfish. / 2031-01-01

Biology

Serotonin

Non-mammalian vertebrates