Ti plasmid and ca mv
SmartKarthi1
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Jul 10, 2017
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About This Presentation
Ti-Plasmid, Genetic transformation Process, episomal expression vectors, DNA viruses
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GENETIC ENGINEERING AND MOLECULAR TECHNIQUES Karthi.M MSc Project Student-Cancer Biology Lab Dept. of Biochemistry
Ti-Plasmid *Tumor-inducing principle – Transferred from the bacterium to the plant at the wound site. * Zaenen at al. (1974) – virulent strains of A.tumefaciens harbor large plasmids (140-235 kbp ) *double stranded circular DNA - Agrobacterium tumefaciens *Agrobacterium is a gram negative soil bacterium - infects over 3000 dicots - causes crown gall disease *This plasmid is denatured at higher temperatures and loses tumorgenic properties.
It encode for enzymes for catabolism of opines such as permease and oxidase
Ti -Plasmid G ene M aps
* Octopine is formed with two amino acids; Arginine and Alanine . * Nopaline is made up of Arginine and Glutamine. * Octopine and nopaline are not found in healthy plant tissues *The opines are catabolized and used as the energy source by the bacterium. *During the infection through a wound, the plant cells begin to proliferate and form tumors and the plant tissues begin to synthesize opines. *It has T DNA which is of 20kb *In addition it has several genes such as vir genes for virulence * ori gene for origin of replication, tra genes for transfer and genes for opine synthesis.
*Virulence gene Responsible for the transfer of T DNA into the host cell and integration of T DNA with host genome * Tra genes encode proteins necessary for transfer of T DNA into the host . *A small, specific segment of the plasmid, about 23kbp in size, is found integrated in the plant nuclear DNA at an apparently random site this DNA segment T-DNA (transferred DNA) *It carries genes that confer both unregulated growth and the ability to synthesize opines upon the transformed plant tissue. *These genes are non-essential for transfer and can be replaced with foreign DNA
*Structure and organization of nopaline plasmid T-DNA sequences are usually simple i.e. there is a single integrated segment * Octopine T-DNA T L (carries the gene required for tumor formation) T R (carries the gene for opine synthesis) *The two segments are transferred to the plant genome independently and may be present as multiple copies *In Ti -plasmid itself T-DNA is flanked by 25 bp imperfect direct repeats border sequences *It is not transferred intact to the plant genome, but they are involved in the transfer process
*Genes in the virulence region are grouped into the virABCDEFG * virA codes for a receptor which reacts to the presence of phenolic compounds such as acetosyringone , which leak out of damaged plant tissues * virB encodes proteins which produce a pore/pilus-like structure * virC binds the overdrive sequence * virD1 and virD2 produce endonucleases which target the direct repeat borders of the T-DNA segment * virE binds to T-strand protecting it from nuclease attack, and intercalates with lipids to form channels in the plant membranes * virG activates vir -gene expression after binding to a consensus sequence once it has been phosphorylated by virA
Genetic transformation Process
* In transferring gene of interest to Ti plasmid, an intermediate vector is used such as pBR 322 . *T DNA portion of the Ti plasmid is separated. T DNA is inserted into the pBR 322 vector which results in formation of a shuttle vector . *This shuttle vector can replicate in E. coli and in Agrobacterium.
Drawback * Ti -plasmid natural vector for genetically engineering plant cells *Because it can transfer its T-DNA from the bacterium to the plant genome *However, wild type Ti -plasmids are not suitable as general gene vectors because the T-DNA contains oncogenes that cause disorganized growth of the recipient plant cells * Deleting all of its oncogene
Plant viruses can be used as episomal expression vectors *Alternative to stable transformation using Agrobac . or d irect DNA transfer, plant viruses can be employed as gene transfer and expression vectors
Advantages to use of Viruses 1 able to adsorb to and introduce their nucleic acid into intact plant cells. However for many viruses, naked DNA or RNA is also infectious, allowing r.combt vec to be introduced directly into plants by methods such as leaf rubbing 2infected cells yield large amt of virus, so r.combt viral vectors have the potential for high-level transgene expression. 3viral infections are often systemic 4viral infections are rapid 5 all known plant viruses replicate episomally
The first plant viral vector were based on DNA viruses Vast majority of plant viruses have RNA genomes. However, two group of DNA viruses that are known to infect plants The caulimoviruses and geminiviruses – 1 st to be developed as vectors because of the ease with which their small, DNA genomes manipulated in plasmid vectors Caulimoviruses – the type member is cauliflower mosaic viruses ( CaMV ). 8 kb dsDNA genome of several isolates has been completely sequenced
Map of the cauliflower mosaic virus genome 8 coding regions Different reading frames DNA strands with the 3 discontinuities Major transcripts – 19s & 35s
Revealing an unusual structure characterised by 3 discontinuities . There are eight tightly packed genes, expressed as two major transcripts 35s RNA (which essentially represents the entire genome), 19s RNA (which contains the coding region for gene VI ) Promoter and terminator sequences for both transcripts have been utilized in plant expression vectors 35s promoter is particularly widely used Only two of the genes in the CaMV genome for non-essential ( gene II & gene VII)
CaMV is icosahedral capsid Max capacity of the CaMV is 8.3kb Removal of all non-essential genes, represents max insert size of less than 1kb This restriction in the capacity for foreign DNA represents a major limitation of CaMV vectors
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