The activity of MSV virion sense promoters and their use in the transformation of cereals

Mazithulela, Gatsha

January 1998

No description available.

630

Genetic transformation of grape somatic embryos

Soloki, Mahmod

January 1997

No description available.

610.28

Development of in vitro and transformation methods for Sorghum bicolor (L. Moench)

17 November 2010

M.Tech. / Sorghum [Sorghum bicolor (L.)] is classified as a relatively recalcitrant crop due to its poor amenability to in vitro and genetic manipulation. An efficient and reproducible in vitro plant regeneration method is vital for a successful transformation of any crop. Plant regeneration and transformation of eight selected elite sorghum genotypes was studied. Immature zygotic embryos were used as explants and cultured on two different callus induction media. Three genotypes ICSV1111N, SRN39 and P898012 were found to be highly regenerable producing 5.99; 5.1 and 4.74 regenerants per explant respectively on the G2+L-proline callus induction medium. The eight elite sorghum genotypes were co-bombarded with the uidA reporter gene and manA selectable marker gene. Bombarded immature zygotic embryos were selected on G2+L-proline callus induction medium supplemented with mannose as a selective agent. PCR Positive transformants were only obtained from genotype P898012. Furthermore the genotype P898012 was stably transformed with a lower DNA amount of manA minimal transgene. The manA gene presence was confirmed with PCR and southern blot analyses and a transformation efficiency of 0.38% was attained. The fertile transgenic plants displayed simple integration patterns, and the gene was also inherited to the T1 progeny of manA resistant trasnsformants in a Mendelian fashion.

Sorghum micropropagation

Sorghum genetic engineering

基因工程倫理課題探討: 消極優生手段對一些嚴重的遺傳病症是一合理及必需的回應. / 消極優生學倫理探討 / Ji yin gong cheng lun li ke ti tan tao: xiao ji you sheng shou duan dui yi xie yan zhong de yi chuan bing zheng shi yi he li ji bi xu de hui ying. / Xiao ji you sheng xue lun li tan tao

January 1991

陳德昌. / Running title: 消極優生學倫理探討. / Thesis (M.Div.)--香港中文大學宗敎及神學學部. / Running title: Xiao ji you sheng xue lun li tan tao. / Includes bibliographical references (leaves 52-61). / Chen Dechang. / Thesis (M.Div.)--Xianggang Zhong wen da xue zong jiao ji shen xue xue bu. / Chapter 一. --- 導 言 --- p.1-6 / Chapter 二. --- 遺傳病理學的發展 --- p.7-12 / Chapter 三. --- 從分配公義的原則看消極優生的必需 --- p.13-21 / Chapter 四. --- 從病者的人生尊嚴看消極優生的必要 --- p.22-25 / Chapter 五. --- 對未來世代的責任 --- p.26-30 / Chapter 六. --- 消極優生手段之産前檢驗的準確性 --- p.31-36 / Chapter 七. --- 基因工程發展與基督教神學思想 --- p.37-50 / Chapter 八. --- 結論 --- p.51 / Chapter 九. --- 附注 --- p.52-61 / Chapter 十. --- 注釋 --- p.62-63 / Chapter 十一. --- 附表 --- p.64-66

The requirement of WHIRLY1 for embryogenesis is dependent on genetic background in maize. / 玉米胚胎發育是否需要WHIRLY1蛋白均定於其所在的遺傳背景 / CUHK electronic theses & dissertations collection / Yu mi pei tai fa yu shi fou xu yao WHIRLY1 dan bai jun ding yu qi suo zai de yi chuan bei jing

January 2013

Zhang, Yafeng. / Thesis (Ph.D.)--Chinese University of Hong Kong, 2013. / Includes bibliographical references (leaves 53-64). / Electronic reproduction. Hong Kong : Chinese University of Hong Kong, [2012] System requirements: Adobe Acrobat Reader. Available via World Wide Web. / Abstracts also in Chinese.

Corn--Genetic engineering

Plant embryology

Gametophytic selection in barley (Hordeum vulgare L.)

Schon, Chris-Carolin

31 May 1990

Graduation date: 1991

Barley -- Genetics

Plant genetic engineering

A MODEL FOR RNA SPLICING OF OVALBUMIN MESSENGER-RNA

Cepits, Judith Diane

January 1982

No description available.

RNA.

Genetic transcription.

Genetic engineering.

Analysis of nodulin-44 gene of soybean

Purohit, Shri Kant.

January 1987

No description available.

Soybean -- Genetics.

Soybean -- Genetic engineering.

Development of novel antibacterial and antiviral transgene vectors and techniques for their application and analysis in sugarcane.

Pepper, Timothy Bryan.

January 2002

Sugarcane is challenged by a number of phytopathogenic bacteria and viruses that are best managed by the development of resistant varieties. Genetic engineering is a promising strategy in such breeding efforts, as it allows novel mechanisms of resistance not available in any parent germplasm to be introduced into the crop. DNA sequences encoding cystatin from papaya (Carica papaya), and pleurocidin from the winter flounder (Pleuronectes americanus) were envisaged as transgenes in this work due to their theoretical potential to increase sugarcane resistance to viruses and pathogenic or opportunistic bacteria, respectively. Cystatin is a cysteine proteinase inhibitor. Cysteine proteinases are used by potyviruses to cleave the polyprotein gene product, an essential step in the viral life cycle. Constitutive expression of cystatin may therefore lend the host plant resistance to a range of potyviruses, including the economically important pathogen sugarcane mosaic virus (SCMV). Pleurocidin is an amphipathic, α-helical, cationic peptide, with broadspectrum anti-bacterial activity at physiological pH. By binding to the cell membranes of both Gram positive and Gram negative bacteria, pleurocidin disrupts the membrane potential, causing it to become more permeable, especially to cations, leading to death of the bacterial cell. Initial microbiological bioassays showed that pleurocidin has inhibitory and bactericidal effects on the organisms which cause leaf scald (Xanthomonas albilineans), gumming disease (Xanthomonas campestris pv. vasculorum) and post-harvest sucrose conversion in sugarcane, as well as inhibitory effects against Leifsonia xyli ssp. xyli, which causes ratoon stunting disease (RSD). For transformation vector construction, the cystatin and pleurocidin coding sequences were altered so that their start codons were in the most favourable consensus context for expression in monocotyledonous plants. In the case of pleurocidin, an extracellular peroxidase signal sequence was attached. The prepared sequences were spliced into the vector pUBI510 in which the gene of interest is driven by the CaMV 35S promoter linked in tandem to a derivative of the maize ubiquitin promoter. The constructs generated were named pUBI510-cys3 and pUBI510-pleur08 respectively. The plasmid structures were confirmed using restriction endonuclease analysis and DNA sequencing. Since the transformation of sugarcane is known to be inefficient, two routes of morphogenesis for the production of somatic embryos were compared in the transformation procedure. These were (1) indirect embryo production via callus and (2) the direct and indirect production of embryos from transverse sections of leaf roll. Field grown sugarcane varieties N12 and NCo376 were the source of explant material. Plasmids pUBI510-cys3 and pUBI510-pleuro8 were respectively co-delivered by microprojectile bombardment with the antibiotic resistance selection plasmid pUBIKN containing the neomycin phosphotransferase gene (npt-II). Cultures were maintained in the dark on selection medium containing various concentrations of the antibiotic geneticin (G418) for several weeks before being allowed to regenerate in the light. Plantlets coming through selection were hardened off in the glasshouse when approximately 100mm high. Primer pairs for amplification of the cystatin insert were designed in various ways. The primer pair which ultimately proved most useful was designed to be complementary to the 5' and 3' ends of the papaya cystatin nucleotide sequence. Primer Premier analysis of a sorghum cystatin sequence provided additional possible primers. A further pair for potential future use was devised based on complementarity to conserved regions on maize cystatins 1 and 2, sorghum, rice, and papaya cystatins. The nucleotide sequence was constructed using the most common monocotyledon codon permutations for each amino acid. Pleurocidin primers were designed to be complementary to 5' and 3' regions of the nucleotide sequence encoding the pleurocidin pre-pro-protein. PCR and RT-PCR protocols for the detection of transgenes and transcript production in putative transgenic plants were developed using these primers. No plants survived selection via the callus route, although some were regenerated via direct embryogenesis. Putative transformed plants were analysed using PCR to test for the presence of integrated transgenes and Southern hybridization to determine transgene copy number. Both types of transgene were reproducibly detectable by PCR in DNA from some immature plants, but results were negative in DNA from those same plants when mature. Southern hybridization analysis detected the cystatin transgene in DNA from immature plants but no transgenes were detected in up to 20 µg DNA from mature plants. Single copy constructions of the transgenes in backgrounds of non-transformed DNA were detectable by both PCR and Southern hybridization analysis. Overall, PCR, RT-PCR and Southern hybridization results indicated that the plants regenerated fell into two categories: non-transformed plants that had survived selection (escapes) and chimaeric individuals with a component of both transformed and non-transformed cells, in which the transgene had probably become diluted during plant development under non-selective conditions. A method for extracting leaf exudates was tested, in conjunction with a cysteine proteinase assay to detect the presence of cystatin transgenes in the intracellular spaces of sugarcane leaves of confirmed transformants. Although it could not be applied within the scope of this project, this assay will prove useful in future work. / Thesis (M.Sc.)-University of Natal, Durban, 2002.

Sugarcane--Genetic engineering.

Theses--Botany.

Heterologous expression of genes in the anaerobic bacterium Streptococcus bovis

Ekinci, Mehmet Sait

January 1997

The main objective of this work was to investigate the expression of xylanase and cellulose genes from <I>Ruminococcus flavefaciens</I> when introduced into related Gram-positive bacteria including the rumen bacterium <I>Streptococcus bovis</I>. In addition the discovery, and isolation of the β(1,3-1,4)-glucanase gene of <I>S. bovis</I> in the course of this work may provide new possibilities to express foreign genes in <I>S. bovis</I> or in other Gram-positive bacteria. The main findings of this work are summarised below: 1. Genes encoding polysaccharidase activity from the strictly anaerobic rumen bacterium <I>R. flavefaciens</I> can be transferred by electroporation into the ruminal bacterium <I>S. bovis</I> and into other Gram-positive bacteria from different habitats, including <I>Lactococcus lactis, Enterococcus faecalis </I>and <I>Streptococcus sanguis</I>. 2. <I>XynD </I>and <I>endA</I> genes of <I>R. flavefaciens </I>can be expressed from their own promoters in these species. Among the bacteria used as hosts for gene expression, <I>S. bovis </I>gave the highest yields of active enzyme. The expression levels of both gene products were found to be higher in <I>S. bovis</I> than in <I>E. coli</I>. 3. The <I>R. flavefaciens </I>enzymes were mainly secreted in the culture medium of <I>S. bovis</I>; however in <I>E. coli</I> they were mainly cell-associated. 4. The full-length enzyme of <I>xynD</I> was detected in several Gram-positive bacteria, suggesting the effect of proteases may be less than in <I>E. coli</I>. 5. The general rearrangement of the introduced plasmid and genes were not found in Gram-positive bacteria and the genes seem to be stable in these organisms. However rearrangement of <I>xynD</I> was observed in some transformants of <I>S. bovis </I>JB1, although non-rearranged transformants were also obtained. 6. Expression of <I>endA</I> and <I>xynD</I> activity was affected by energy sources supplied to <I>S. bovis</I> cultures, reflecting the accumulation of lactic acid.

572.8

Rumen bacteria; Genetic engineering