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21	Isolation and characterization of oat seed globulin and synthesis of oat seed storage proteins Brinegar, Anthony Chris. January 1983 (has links) Thesis (Ph. D.)--University of Wisconsin--Madison, 1983. / Typescript. Vita. eContent provider-neutral record in process. Description based on print version record. Includes bibliographical references (leaves 116-126). Oats Globin. Proteins.
22	The role of histone deacetylase 10 in y-globin gene regulation / Nimer, Sadeieh Abedaljaleel, January 2008 (has links) Thesis (M.S.)--University of Texas at Dallas, 2008. / Includes vita. Non-Latin script record Includes bibliographical references (leaves 39-40) Histone deacetylase. Globin genes.
23	The Role of GLP Domains in Spreading of the G9a/GLP Complex and Regulation of the β-globin Gene Expression Thieba, Camilia Annik January 2012 (has links) Marked by a defect in the production of the Beta (β)-globin chain that make-up hemoglobin, Beta (β)-thalassemia is the most prevalent form of inherited single-gene disorders in the world. To understand the molecular mechanisms that govern the expression of the β-globin polypeptide encoded by the β-globin locus, we examined closely the enzymes involved in the epigenetic regulation of gene expression through histone 3 lysine 9 mono and di-methylation (H3K9 me1/2). G9a-like protein (GLP), a mammalian methyltransferase involved in the establishment and maintenance of H3K9 me1/2 mark at euchromatin, regions was found to be critical for the full activation of the adult β-globin genes in vivo during Murine erythroleukemia cell line (MEL) differentiation. Though it was initially hypothesized that GLP binding to H3K9 me1/2 mark through its Ankyrin domain was key to its activating function, we found that Flag- GLP ankyrin mutants E817R and W791A unable to bind to the methyl mark, are able to activate β-globin genes as well as their wild-type counterpart. Additionally, this study found that the embryonic gene εγ, known to be re-activated after G9a KD at the mRNA level, was effectively transcribed at the protein level using Triton Urea Acetic acid (TAU) western blots, thereby identifying potential therapeutic applications for treatment for β-thalassemia patients. GLP G9a chromatin globin
24	Regulatory and functional study of human cytoglobin Guo, Xiumei, 郭秀梅 January 2007 (has links) published_or_final_version / abstract / Biological Sciences / Doctoral / Doctor of Philosophy Globin - Synthesis - Regulation. Globin genes - Expression. Oxidative stress.
25	Genomic isolation and molecular analysis of a rat [alpha]-globin gene cluster 馬忠華, Ma, Chung-wah. January 1998 (has links) published_or_final_version / Biochemistry / Doctoral / Doctor of Philosophy Globin genes. Molecular cloning. Rats.
26	Molecular characterization of the mouse cytoglobin Chow, Kwok-fai, Joseph, 周國輝 January 2006 (has links) published_or_final_version / abstract / Zoology / Doctoral / Doctor of Philosophy Globin. Genomes. Mice - Molecular aspects.
27	Transcription factors regulating the human beta-globin genes Wrighton, N. C. January 1988 (has links) No description available. 572.8 Gene expression/human globin
28	Detection of clinically silent beta-globin gene mutations in Chinese using high resolution melting analysis Tsang, Ho-yin, 曾皓言 January 2012 (has links) Mutations in the beta-globin (β-globin) gene cause beta-thalassaemia (β-thalassaemia).The screening strategy for β-thalassaemiais based on the value of mean corpuscular volume (MCV) from the complete blood count (CBC) data. Current laboratory practice considers blood samples with MCV higher than 80fL as normal. No further assessment will be done on these samples. However, there are clinically silent β-globin gene mutations with MCV higher than 80fL, for example, heterozygous haemoglobin E (HbE). The importance of finding out this kind of mutations is due to the serious outcome when they occur together with classic β thalassaemia mutations in compound heterozygous states, which may produce a condition mimicking β thalassaemia major. The method used to recognize the presence of clinically silent β-globin gene mutations should be robust and with high sensitivity. High resolution melting (HRM) is a suitable technique to screen gene mutations. It is fast and convenient. The process is completed in a closed system without any post PCR manipulation. The sensitivity is up to a single nucleotide change. Using HRM for mutations screening followed by confirmation with sequencing can reduce time and cost of testing clinically silent β-globin gene mutations on a large scale. This study first shows the ability of HRM in detecting various types of β-globin gene mutations. The technique is then applied to detect clinically silent β-globin gene mutations in a group of high school students with normal CBC data. Mutations with different clinically significance were found. The frequency of mutation found in the samples of the study suggests that screening for β-globin gene mutation may be worthwhile in subjects with MCV higher than 80fL. / published_or_final_version / Pathology / Master / Master of Medical Sciences Thalassemia - Genetic aspects. Globin genes.
29	Detection of uncommon globin gene mutations causing unexplained microcytosis in Chinese Liu, Ka-wun, Ada., 劉嘉媛. January 2012 (has links) The thalassaemias are the commonest monogenic disorders in the world population. They occur at a particularly high frequency in Mediterranean regions and Southeast Asia, which cause a massive public health problem. In Hong Kong, the prevalence of heterozygous carriers of α or β thalassaemia mutations is approximately 8% [1]. Thalassaemia is characterized by the reduced synthesis of one or more normal globin chains. This causes globin chain imbalance and finally leads to hypochromic microcytic anaemia. Different types of thalassaemia are named according to the under-produced chains. The majority of thalassaemia can be diagnosed by basic haematologic profiles and simple phenotypic techniques. However, in some cases of thalassaemia the diagnosis are not apparent after routine laboratory investigations. To arrive at a diagnosis which is important for antenatal diagnosis and genetic counseling, it is necessary to use molecular approaches. In this study, 25 patients with microcytosis, normal phenotypic haemoglobin study results and without iron deficiency were analyzed retrospectively. This cohort of patients was suspected to have occult or masked thalassaemia. DNA was extracted from archive samples and further investigated by alpha multiplex gap polymerase chain reaction (α multiplex gap-PCR), alpha amplification refractory mutation system (α ARMS) and direct nucleotide sequencing of globin genes for the detection of possible underlying globin gene mutations. Results indicated that 60% of these cases with microcytosis were occult and silent αthalassaemia caused by deletional or non-deletional mutations. Maskedβthalassaemia due to co-existing δ thalassaemia or variants or normal Hb A2 β thalassaemia due to mild β globin gene mutations were not detected in the cohort. Forty percent of these cases of microcytosis remained unexplained, which await further molecular testing. / published_or_final_version / Pathology / Master / Master of Medical Sciences Thalassemia - Genetic aspects. Globin genes.
30	Molecular analysis of the -globin gene cluster among the Chinese population 廖永新, Liu, Wing-sun, Vincent. January 1986 (has links) published_or_final_version / Medicine / Master / Master of Philosophy Globin. Human population genetics - China.

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