Global ETD Search

1	Deer (cervus elaphus) epidermal growth factor-like activity. January 1986 (has links) by Kam-ming Ko. / Includes bibliographical references / Thesis (M.Ph.)--Chinese University of Hong Kong, 1986 Deer--Growth Antlers--Growth Growth--Research
2	The microaerophilic nature of <i>Wolinella recta, Wolinella curva, Bacteroides ureolyticus</i>, and <i>Bacteroides gracilis</i> Han, Yeong-Hwan 10 October 2005 (has links) Broad relationships among bacteria can be identified by ribosomal RNA analysis, but the resulting groups may not be easily definable by phenotypic characteristics. This is exemplified by the genus <i>Campylobacter</i>, which consists of at least three separate groups that cannot be differentiated readily by phenotypic characteristics. Examination of the type strains of all Campylobacter species (except <i>Campylobacter pylori), Wolinella recta, Wolinella curva, Bacteroides ureolyticus</i>, and <i>Bacteroides gracilis</i> revealed that sheathed flagella occur only in species of rRNA group II (except <i>W.succinogenes</i>). This is helpful in differentiating this group. Campylobacters are microaerophilic: they can respire with oxygen but cannot grow at the full level of oxygen found in an air atmosphere (21% O₂). Although <i>W. recta, W. curva, B. ureolyticus</i>, and <i>B. gracilis</i> are closely related to the campylobacters of rRNA group I, they were thought to be anaerobes, incapable of oxygen-dependent growth and of respiring with O₂. However, the present study revealed that they are in fact microaerophiles. They exhibited oxygen-dependent growth but failed to grow at 21% O₂ and grew only very slightly under anaerobic conditions unless provided with electron acceptors such as fumarate and nitrate. They exhibited 0₂ uptake with H₂ or formate as electron donors (<i>W. recta</i> showed only a low O₂ uptake with H₂). Oxygen uptake was inhibited by KCN and 2-heptyl-4-hydroxyquinoline N-oxide. The organisms possessed membrane bound cytochromes (cytochromes b560 and C551-553, and a CO-binding cytochrome c), as well as soluble cytochrome C552 and CO-binding cytochrome c. The cytochromes were reduced by H₂ and formate as electron donors. Proton efflux from cells in anaerobic suspensions containing H₂ or formate occurred upon addition of a pulse of oxygen. With formate as the electron donor, H+/O ratios of <i>W. curva, W. recta, B. ureolyticus</i>, and <i>B. gracilis</i> were 0.75, 1.66,2.06, and 2.04, respectively. With H₂ as the electron donor, H⁺/O ratios of <i>W.curva, B. ureoyticus, and B. gracilis</i> were 1.25, 1.97, and 2.36, respectively; technical difficulties prevented measurement of the ratio in <i>W. recta</i>. Proton translocation was inhibited by the protonophore carbonylcyanide <i>m</i>-chlorophenylhydrazone. The results confirm the relationship of these organisms to campylobacters. / Ph. D. LD5655.V856 1991.H373 Bacteria -- Research Bacterial growth -- Research
3	Osteo-inductive potential of different doses of recombinant human osteogenic protein-1 Odendaal, Petrus Johannes 05 January 2007 (has links) Please read the abstract in the section 00front of this document / Dissertation (MChD (Periodontics and Oral Medicine))--University of Pretoria, 2007. / Oral Pathology and Oral Biology / unrestricted Bone regeneration research Bones growth research Periodortics research Gingivitis prevention Teeth care and hygiene UCTD
4	Shoot apex culture of Acacia mearnsii (De wild) Thompson, Iain Mungo. January 2007 (has links) Research into the micropropagation of black wattle in South Africa is important for two reasons. Firstly micropropagation technology allows breeders to select and propagate mature tissue, which in turn allows them to better capture selected traits. Secondly, tissue culture may control the highly invasive nature of black wattle. If triploid black wattle can be developed, foresters will then have to rely on clonal propagation to supply material for their growing operations. This research was part of the Institute for Commercial Forestry’s Acacia mearnsii vegetative propagation programme. The main focus of this research was to overcome various problems associated with direct organogenesis of ex vitro material. The shoot apex region was used as the explant in all studies because this region is thought to harbour relatively few internal microbial contaminants and is of sufficient size to withstand stresses associated with micropropagation. The initial research was focussed on the screening of sterilants, searching for a viable alternative to mercuric chloride. Surface sterilisation is integral to any micropropagation technique. This process should do the least amount of plant damage, whilst reducing microbial contamination to an acceptable level. Explants were cultured on Murashige and Skoog (MS) medium supplemented with 2.0 mg L-1 BA and monitored for signs of contamination and shooting. Household bleach proved an excellent alternative to mercuric chloride because it did significantly less damage to the explants than mercuric chloride and is handled easily. There was no significant effect of sterilant exposure time on explant decontamination levels, whilst the shortest exposure time resulted in significantly higher levels of shoot development than the other two times tested. The results of this initial research was developed into a protocol and utilised in subsequent investigations. Due to a considerable variation in the success of the developed surface sterilisation protocol according to different times of the year, a further investigation into the effects of season and mother plant material on shoot apex culture of Acacia mearnsii was undertaken. The success of any tissue culture technique depends on a large array of ex vitro and in vitro variables. The objective of this research was to determine the ii effect of two ex vitro variables, season and mother plant, on shoot apex culture of Acacia mearnsii. Explants from individual mother plants were cultured on MS medium supplemented with 2.0 mg L-1 BA during four separate seasons and monitored for signs of contamination and shooting. Spring was found to be the best harvesting season because spring explants showed significantly higher decontaminated explant levels and shooting levels than explants harvested in the other three seasons. The effect of mother plant selection on the performance of Acacia mearnsii explants during shoot apex culture was also found to be significant, especially with regard to shooting levels. Finally factors influencing shoot elongation of A. mearnsii during shoot apex culture were investigated. In the past, induction of shoot elongation during micropropagation of A. mearnsii was attained through the addition of plant growth regulators and other supplements to the basal culture medium. However, some micropropagation methods in other species have utilised red light as a means of promoting shoot elongation. The objective of this study was to test the effects of an alternative basal medium, red light and differing concentrations of chemical additions to the culture medium on shoot elongation of Acacia mearnsii during shoot apex culture. Four independent experiments were undertaken comparing: shoot elongation on Woody Plant Medium (WPM) to the MS basal medium control; shoot elongation under a red cellophane box compared to control culture light conditions; shoot elongation on media supplemented with various concentrations of GA3 to the un-supplemented control and shoot elongation on media supplemented with combinations of BA and IBA compared to a control. Although no significant effects were observed, many trends were noted. The results indicated that there was no advantage to using WPM instead of MS medium when attempting to elongate shoots, rejuvenated through shoot apex culture of A. mearnsii, whilst the effect of GA3 showed a negative trend. The effects of red light and some BA and IBA combinations showed positive trends on the elongation of initiated shoots. This research successfully addressed some of the problems associated with micropropagation of A. mearnsii. Shoot apex culture shows promise and further research into this technique should be considered. A viable surface sterilant alternative to mercuric chloride was successfully identified. This alternative is not only iii safer to use but shows a large reduction in phytotoxic effects. The effects of season and mother plant on shoot apex culture was successfully investigated, resulting in a better understanding of mother plant influences on tissue culture as well as the identification of an optimum season for explant selection. Finally two possible shoot elongation promoters were identified for further research and a more affordable alternative to red light sources and screens was identified. / Thesis (M.Sc.)-University of KwaZulu-Natal, Pietermaritzburg, 2007. Acacia mearnsii. Plant tissue culture. Acacia mearnsii--Micropropagation. Acacia mearnsii--Growth--Research. Wattles (Plants)--Propagation. Acacia mearnsii--Propagation. Acacia mearnsii--Research--South Africa. Plant micropropagation. Theses--Plant pathology.
5	The function of ASCL1 in pregnancy-induced maternal liver growth Lee, Joonyong January 2014 (has links) Indiana University-Purdue University Indianapolis (IUPUI) / The maternal liver shows marked growth during pregnancy to accommodate the development and metabolic needs of the placenta and fetus. Previous study has shown that the maternal liver grows proportionally to the increase in body weight during gestation by hyperplasia and hypertrophy of hepatocytes. As the maternal liver is enlarged, the transcript level of Ascl1, a transcription factor essential to progenitor cells of the central nervous system and peripheral nervous system, is highly upregulated. The aims of the study were to (1) identify hepatic Ascl1-expressing cells, and (2) study the functions of Ascl1 in maternal liver during pregnancy. In situ hybridization shows that most cell types (parenchymal, nonparenchymal, and mesothelial cells) express Ascl1 mRNA in maternal livers during gestation and in male regenerating livers. Notably, hepatic mesothelial cells abundantly express Ascl1 during pregnancy and liver regeneration. Inducible ablation of Ascl1 gene during pregnancy results in maternal liver enlargement, litter size reduction, and fetal growth retardation. In addition, maternal hepatocytes deficient in Ascl1 gene lack majority of their cytosols and exhibit β-catenin nuclear translocation, while maintaining their cellular boundary and identity. In summary, in both maternal liver during pregnancy and regenerating liver, the expression of Ascl1 is induced in most cell types. Mesothelial cells are potential origin of Ascl1-expressing cells. Ascl1 gene is essential for the progression of normal pregnancy Pregnancy -- Research Hepatocyte growth factor -- Research Liver -- Growth -- Research Maternal-fetal exchange Hyperplasia Liver -- Hypertrophy Gene expression -- Research Developmental neurobiology Fetal liver cells Liver -- Regeneration Stem cells -- Research Nerves, Peripheral
6	Identification and characterization of Ascl1-expressing cells in maternal liver during pregnancy Kumar, Sudhanshu 01 August 2014 (has links) Indiana University-Purdue University Indianapolis (IUPUI) / During pregnancy, maternal liver exhibits robust growth to meet the metabolic demands of the developing placenta and fetus. Although hepatocyte hypertrophy and hyperplasia are seen in the maternal liver, the molecular and cellular mechanisms mediating the maternal hepatic adaptations to pregnancy is poorly understood. Previous microarray analysis revealed a most upregulated gene named Ascl1, a transcription factor essential for neural development, in the maternal liver at mid-gestation. The aims of the study were to (1) validate the activation of Ascl1 gene; (2) identify Ascl1-expressing cells; and (3) determine the fate of Ascl1-expressing cells, in the maternal liver during the course of gestation. Timed pregnancy was setup in mice and the maternal livers were collected at various stages of gestation. Maternal hepatic Ascl1 mRNA expression was evaluated by qRT-PCR and northern blotting. The results demonstrated that the transcript level of maternal hepatic Ascl1 is exponentially increased during the second half of pregnancy in comparison with a non-pregnant state. Using a Ascl1-GFP mouse model generated by others to monitor the behavior of neural progenitor cells, we found that maternal hepatic Ascl1-expressing cells are non-parenchymal cells, very small in size, and expanding during pregnancy. To map the fate of this cell population, we generated an in vivo tracing mouse model named Ascl1-CreERT2/ROSA26-LacZ. Using this model, we permanently labeled maternal hepatic Ascl1-expressing cells at midgestation by giving tamoxifen and analyzed the labeled cells in the maternal liver prior to parturition. We observed that the initial small Ascl1-expressing cells undergoing expansion at mid-gestation eventually became hepatocyte-like cells at the end stage of pregnancy. Taken together, our findings strongly suggest that Ascl1-expressing cells represent a novel population of hepatic progenitor cells and they can differentiate along hepatocyte lineage and contribute to pregnancy-induced maternal liver growth. Further studies are needed to firmly establish the nature and property of maternal hepatic Ascl1-expressing cells. At this stage, we have gained significant insights into the cellular mechanism by which the maternal liver adapts to pregnancy. Ascl1 Liver Regeneration Pregnancy Pregnancy in animals -- Research Liver -- Regeneration -- Research Liver -- Growth -- Research Liver -- Anatomy Liver cells -- Differentiation DNA microarrays -- Research Gene expression -- Research Hepatocyte growth factor -- Research Protein microarrays Developmental neurobiology Tamoxifen -- Research
7	Lineage tracing of Ascl1-expressing cells in the maternal liver during pregnancy Nambiar, Shashank Manohar January 2014 (has links) Indiana University-Purdue University Indianapolis (IUPUI) / To cope with the high metabolic demands of the body during pregnancy, the maternal liver adapts by increasing its mass and size. This increase is proportional to the increase in total body weight during the course of gestation. The pregnancy-induced maternal liver growth is a result of both hepatocyte hypertrophy and hyperplasia. Microarray analysis of pregnant maternal livers shows markedly different gene expression profiles when compared to a non-pregnant state. Most interesting was the 2,500-fold up-regulation in the mRNA expression of Ascl1, a transcription factor responsible for the differentiation of neural progenitor cells into various neuronal types, during the second half of pregnancy. Our investigation aimed at (1) characterizing the identity of maternal hepatic Ascl1-expressing cells and (2) tracing the fate of Ascl1-expressing cells in the maternal liver during pregnancy. Timed pregnancies were generated and non-pregnant (NP) and pregnant maternal livers were harvested and analysed. To identify the maternal hepatic Ascl1-expressing cells we used the Ascl1GFP/+ reporter mouse line. NP and gestation day 15 (D15) maternal livers were immunostained for green fluorescent protein (GFP). The result shows that GFP-positive, Ascl1-expressing cells are hepatocyte-like cells, which are present in D15 maternal livers, but absent in NP livers. The Rosa26floxstopLacZ/ floxstopLacZ;Ascl1CreERT2/+ mouse line was used to trace the fate of Ascl1-expressing cells during pregnancy. LacZ staining of gestation day 13 (D13) and 18 (D18) maternal livers demonstrates that D13 hepatic Ascl1-expressing cells (labeled with LacZ) undergo hyperplasia to repopulate a large portion of D18 maternal livers. Furthermore, LacZ and HNF4α co-staining of D13 and D18 maternal livers shows the presence of two populations of LacZ-expressing cells: HNF4α+ population and HNF4α- population. HNF4α+ LacZ-expressing cells represent hepatocyte lineage cells that are derived from Ascl1-expressing cells. We observe that, towards the end of pregnancy, a considerable portion of the maternal liver is comprised of hepatocytes derived from Ascl1-expressing cells. Taken together, our preliminary study suggests that pregnancy induces maternal liver turnover via Ascl1-expressing cells. Liver -- Growth -- Research Hyperplasia -- Research Gene expression -- Research Pregnancy -- Research Liver -- Regeneration Neural stem cells -- Research Messenger RNA Stem cells -- Research Animal models in research
8	The essential role of Stat3 in bone homeostasis and mechanotransduction Zhou, Hongkang January 2014 (has links) Indiana University-Purdue University Indianapolis (IUPUI) / Signal Transducer and Activator of Transcription 3 (Stat3) is a transcription factor expressed in bone and joint cells that include osteoblasts, osteocytes, osteoclasts, and chondrocytes. Stat3 is activated by a variety of cytokines and growth factors, including IL-6/gp130 family cytokines. These cytokines not only regulate the differentiation of osteoblasts and osteoclasts, but also regulate proliferation of chondrocytes through Stat3 activation. In 2007, mutations of Stat3 have been confirmed to cause a rare human immunodeficiency disease – Job syndrome which presents skeletal abnormalities like: reduced bone density (osteopenia), scoliosis, hyperextensibility of joints, and recurrent pathological bone fractures. Changes in the Stat3 gene alter the structure and function of the Stat3 proteins, impairing its ability to control the activity of other genes. However, little is known about the effects of Stat3 mutations on bone cells and tissues. To investigate the in vivo physiological role of Stat3 in bone homeostasis, osteoblast/osteocyte-specific Stat3 knockout (KO) mice were generated via the Cre-LoxP recombination system. The osteoblast/osteocyte-specific Stat3 KO mice showed bone abnormalities and an osteoporotic phenotype because of a reduced bone formation rate. Furthermore, inactivation of Stat3 decreased load-driven bone formation, and the disruption of Stat3 in osteoblasts suppressed load-driven mitochondrial activity, which led to an elevated level of reactive oxygen species (ROS) in cultured primary osteoblasts. Stat3 has been found to be responsive to mechanical stimulation, and might play an important role in mechanical signal transduction in osteocytes. To investigate the role Stat3 plays in mechanical signaling transduction, osteocyte-specific Stat3 knockout (KO) mice were created. Inactivation of Stat3 in osteocytes presented a significantly reduced load-driven bone formation. Decreased osteoblast activity indicated by reduced osteoid surface was also found in osteocyte-specific Stat3 KO mice. Moreover, sclerostin (SOST) protein which is a critical osteocyte-specific inhibitor of bone formation, its encoded gene SOST expression has been found to be enhanced in osteocyte-specific Stat3 KO mice. Thus, these results clearly demonstrated that Stat3 plays an important role in bone homeostasis and mechanotransduction, and Stat3 is not only involved in bone-formation-important genes regulation in the nucleus but also in mediation of ROS and oxidative stress in mitochondria. Bone formation Osteoblast Osteocyte Mechanotransduction Bones -- Growth -- Molecular aspects Human mechanics Bones -- Physiology Biomechanics -- Research Bones -- Metabolism -- Disorders Osteocytes -- Research Osteoblasts -- Research Osteoclasts -- Research Bone cells -- Research Cellular signal transduction -- Research Transcription factors -- Research Bone remodeling
9	Hand2 function within non-cardiomyocytes regulates cardiac morphogenesis and performance VanDusen, Nathan J. January 2014 (has links) Indiana University-Purdue University Indianapolis (IUPUI) / The heart is a complex organ that is composed of numerous cell types, which must integrate their programs for proper specification, differentiation, and cardiac morphogenesis. During cardiac development the basic helix-loop-helix transcription factor Hand2 is dynamically expressed within the endocardium and extra-cardiac lineages such as the epicardium, cardiac neural crest cells (cNCCs), and NCC derived components of the autonomic nervous system. To investigate Hand2 function within these populations we utilized multiple murine Hand2 Conditional Knockout (H2CKO) genetic models. These studies establish for the first time a functional requirement for Hand2 within the endocardium, as several distinct phenotypes including hypotrabeculation, tricuspid atresia, aberrant septation, and precocious coronary development are observed in endocardial H2CKOs. Molecular analyses reveal that endocardial Hand2 functions within the Notch signaling pathway to regulate expression of Nrg1, which encodes a crucial secreted growth factor. Furthermore, we demonstrate that Notch signaling regulates coronary angiogenesis via Hand2 mediated modulation of Vegf signaling. Hand2 is strongly expressed within midgestation NCC and endocardium derived cardiac cushion mesenchyme. To ascertain the function of Hand2 within these cells we employed the Periostin Cre (Postn-Cre), which marks cushion mesenchyme, a small subset of the epicardium, and components of the autonomic nervous system, to conditionally ablate Hand2. We find that Postn-Cre H2CKOs die shortly after birth despite a lack of cardiac structural defects. Gene expression analyses demonstrate that Postn-Cre ablates Hand2 from the adrenal medulla, causing downregulation of Dopamine Beta Hydroxylase (Dbh), a gene encoding a crucial catecholaminergic biosynthetic enzyme. Electrocardiograms demonstrate that 3-day postnatal Postn-Cre H2CKO pups exhibit significantly slower heart rates than control littermates. In conjunction with the aforementioned gene expression analyses, these results indicate that loss of Hand2 function within the adrenal medulla results in a catecholamine deficiency and subsequent heart failure. Hand2 Cardiac Development Tricuspid Atresia Endocardium Notch Signaling EphrinB2 bHLH Transcription Factor Tricuspid valve -- Research Endocardium -- Research Neural crest Helix-loop-helix motifs -- Research Transcription factors Notch genes Cellular signal transduction -- Research Cell receptors Gene expression Heart cells Protein-tyrosine kinase Autonomic nervous system -- Physiology Heart conduction system Notch proteins Morphogenesis -- Molecular aspects

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