Making transgenic plants 1.Identify and clone DNA sequence encoding desired protein into suitable vector = DNA molecule that allows sequence to be propagated.

Slides:

Advertisements

Similar presentations

Plant Genetic Transformation. All stable transformation methods consist of three steps: Delivery of DNA into a single plant cell. Integration of the DNA.

Advertisements

Genetic Engineering of Plants BIT 220 End of Chapter 22.

DNA Technology & Gene Mapping Biotechnology has led to many advances in science and medicine including the creation of DNA clones via recombinant clones,

Lecture 8 Genetic Engineering. Medically important substances produced by genetic engineering Human Insulin- used to treat diabetes Past: extracted insulin.

Cloning Promoters Kelli Henry April 27, 2009.

Plan A Topics? 1.Making a probiotic strain of E.coli that destroys oxalate to help treat kidney stones in collaboration with Dr. Lucent and Dr. VanWert.

Ti plasmid derived vector system

Recombinant DNA, Biotechnology, and Microbes Microbiology 221.

 Intent of altering human genome  Introducing new genetic material into genome  Insulin.

CHAPTER 31 Genetic Engineering and Biotechnology.

Transformation/Transfection

Genetic Engineering learning outcomes

Lecture 10 Chapter 7 Recombinant DNA, Vector Design and Construction Neal Stewart.

Next Assignment = GMO plants

Agrobacterium tumefaciens

Genetics and Genetic Engineering terms clones b organisms or cells of nearly identical genetic makeup derived from a single source.

CHAPTER 20 BIOTECHNOLOGY: PART I. BIOTECHNOLOGY Biotechnology – the manipulation of organisms or their components to make useful products Biotechnology.

Genetic Engineering Intent of altering human genome

Genetic Engineering Regular Biology. Selective Breeding  This is the process of allowing those organisms with specific characteristics to reproduce 

Ms. Gaynor Honors Genetics Biotechnology and the Use of Bacteria.

Chapter 18-Genetic Engineering of Plants: Methodology

© 2012 Pearson Education, Inc. Lecture by Edward J. Zalisko PowerPoint Lectures for Campbell Biology: Concepts & Connections, Seventh Edition Reece, Taylor,

PLANT VECTORS REKHA PULICHERLA

AP Biology Biotechnology Part 3. Bacterial Cloning Process Bacterium Bacterial chromosome Plasmid Gene inserted into plasmid Cell containing gene of interest.

TEST 4 review. _____ 1. A prophage is a(n) a. emerging virus. b. type of retrovirus. c. prion that has been integrated into a bacterial cell's chromosome.

Genetically Modified Organisms (GMOs) Any microorganism, plant or animal that has purposely had its genome altered using genetic engineering technology.

Human awareness.  M16.1 Know that the DNA can be extracted from cells  Genetic engineering and /or genetic modification have been made possible by isolating.

DNA Manipulation 2. DNA The nucleus contains DNA.

Cloning Genes Gene cloning: amplifying a specific piece of DNA via a bacteria cell Cloning vector: a replicating DNA molecule attached with a foreign DNA.

Next Assignment = GMO plants In class starting March 27 Herbicide resistance Bromoxynil Glyphosate (roundup) Glufosinate (Basta) Isoxaflutole (Balance,

© SSER Ltd.. Gene Technology or Recombinant DNA Technology is about the manipulation of genes Recombinant DNA Technology involves the isolation of DNA.

Plant Tissue Culture collection of techniques used to maintain or grow plant cells, tissues, or organs under sterile conditions mostly used to produce.

Course Project = Algal Lipid Production

Relationship between Genotype and Phenotype

Studying the genomes of organisms GENE TECHNOLOGY.

Plasmids and Vectors Aims:

Gene delivery techniques

Chapter 20: Part 1 DNA Cloning and Plasmids

1 DNA and Biotechnology. 2 Outline DNA Structure and Function DNA Replication RNA Structure and Function – Types of RNA Gene Expression – Transcription.

Light-independent (dark) reactions occur in the stroma of the chloroplast (pH 8) Consumes ATP & NADPH from light reactions regenerates ADP, Pi and NADP.

CHAPTER 20 BIOTECHNOLOGY. Biotechnology – the manipulation of organisms or their components to make useful products Biotechnology is used in all facets.

Agrobacterium tumefaciens The Journey from Plant Pathology to Biotechnology Bonnie Ownley Entomology and Plant Pathology University of Tennessee, Knoxville.

Genetic Engineering. Entire organisms can be cloned  Clone  a genetically identical copy of a gene or of an organism  Cloning occurs in nature:  Bacteria.

Bacterial Transformation Green Fluorescent Protein.

Genetic Engineering of Plants Must get DNA: 1.into the cells 2.integrated into the genome (unless using transient expression assays) 3.expressed (everywhere.

VECTORS: TYPES AND CHARACTERISTICS

Principles of genetic engineering. OBJECTIVE To describe the main stages in genetic engineering.

Recombinant DNA and Gene Cloning

Introduction to Biotechnology Transformation and more!

4/26/2010 BIOTECHNOLOGY.

V Cell Transformation Recombinant DNA Host Cell DNA Target gene

Molecular Genetic Analysis and Biotechnology

Chapter 10 – Genetic Engineering of Plants: Methodology

13-3 Cell Transformation Interactive pgs. 329.

Topics? Trying to find another way to remove oxalate

Arrangements Forensic uses

Topics? Trying to find another way to remove oxalate

Biotechnology: Part 1 DNA Cloning, Restriction Enzymes and Plasmids

BIO201 Introduction to Biochemistry & Biotechnology

Chapter 14 Bioinformatics—the study of a genome

Chapter 13.3 Cell Transformation.

4/26/2010 BIOTECHNOLOGY.

Genetic Engineering pp

CHAPTER 20 DNA TECHNOLOGY.

TOOLS OF BIOTECHNOLOGY

Metabolism and Survival

Cell Transformation.

GENE TECHNOLOGY Chapter 13.

Plasmids circular pieces of”extrachromosomal” DNA propagated inside host have origin of replication -> ensures host will copy it.

Lipid metabolism Unique aspects in plants Make fatty acids by

Presentation transcript:

Making transgenic plants 1.Identify and clone DNA sequence encoding desired protein into suitable vector = DNA molecule that allows sequence to be propagated in chosen host create a recombinant DNA molecule

Making transgenic plants 1) create recombinant DNA 2) transform recombinant molecules into suitable host

Making transgenic plants 1) create recombinant DNA 2) transform recombinant molecules into suitable host 3) identify hosts which have taken up your recombinant molecules

Making transgenic plants 1) create recombinant DNA 2) transform recombinant molecules into suitable host 3) identify hosts which have taken up your recombinant molecules 4) Confirm they contain the recombinant DNA

Making transgenic plants 1.Identify and clone DNA sequence encoding desired protein into suitable vector = DNA molecule with: Origin of replication that functions in chosen host “Selectable marker” = gene encoding protein allowing selection of hosts that have taken up the recombinant molecule Cloning site = dispensable region where foreign DNA can be inserted

Making transgenic plants 1.Identify and clone DNA sequence encoding desired protein into suitable vector = DNA molecule with: Origin of replication that functions in chosen host “Selectable marker” = gene encoding protein allowing selection of hosts that have taken up the recombinant molecule Cloning site = dispensable region where foreign DNA can be inserted

Making transgenic plants 1.Identify and clone DNA sequence encoding desired protein into suitable vector 2.Vectors for plant transformation add promoters, terminators and selectable markers that work in plant cells

Making transgenic plants 1.Digest DNA and vector with same restriction enzyme Assume have identified the DNA sequence to clone, eg by PCR

Making transgenic plants 1.Digest DNA and vector with same restriction enzyme 2.Allow them to anneal, then seal nicked backbone with DNA ligase

Making transgenic plants 1.Digest DNA and vector with same restriction enzyme 2.Allow them to anneal, then seal nicked backbone with DNA ligase 3.Transform into bacteria

Making transgenic plants 1.Digest DNA and vector with same restriction enzyme 2.Allow them to anneal, then seal nicked backbone with DNA ligase 3.Transform into bacteria 4.Extract plasmid

Making transgenic plants 1.Digest DNA and vector with same restriction enzyme 2.Allow them to anneal, then seal nicked backbone with DNA ligase 3.Transform into bacteria 4.Extract plasmid 5.Directly add to plants or transfer to Agrobacterium tumefasciens

Making transgenic plants 1.Digest DNA and vector with same restriction enzyme 2.Allow them to anneal, then seal nicked backbone with DNA ligase 3.Transform into bacteria 4.Extract plasmid 5.Directly add to plants or transfer to Agrobacterium tumefasciens 6.Select transgenics

Agrobacterium tumefasciens (Rhizobium radiobacter) Gram-negative pathogenic soil bacterium of Rhizobiaceae (same family as Rhizobium symbionts)

Agrobacterium tumefasciens (Rhizobium radiobacter) Gram-negative pathogenic soil bacterium of Rhizobiaceae (same family as Rhizobium symbionts) Causes crown galls in over 140 dicot plant spp.

Agrobacterium tumefasciens (Rhizobium radiobacter) Gram-negative pathogenic soil bacterium of Rhizobiaceae (same family as Rhizobium symbionts) Causes crown galls in over 140 plant spp. Contains 206,000 bp Tumor-inducing (Ti) plasmid

Agrobacterium tumefasciens (Rhizobium radiobacter) Contains 2006,000 bp Tumor-inducing (Ti) plasmid When infects host transfers T-DNA (from left to right border of Ti plasmid) that inserts into host chromosome

Agrobacterium tumefasciens (Rhizobium radiobacter) Contains 2006,000 bp Tumor-inducing (Ti) plasmid When infects host transfers T-DNA (from left to right border of Ti plasmid) that inserts into host chromosome Process resembles conjugation

Agrobacterium tumefasciens (Rhizobium radiobacter) When infects host transfers T-DNA (from left to right border of Ti plasmid) that inserts into host chromosome Process resembles conjugation T-DNA contains “oncogenic genes” that cause overproduction of auxin and cytokinin

Agrobacterium tumefasciens (Rhizobium radiobacter) When infects host transfers T-DNA (from left to right border of Ti plasmid) that inserts into host chromosome Process resembles conjugation T-DNA contains “oncogenic genes” that cause overproduction of auxin and cytokinin: make transformed cells form tumors

Agrobacterium tumefasciens (Rhizobium radiobacter) T-DNA contains “oncogenic genes” that cause overproduction of auxin and cytokinin: cause transformed cells to form tumors Also have gene forcing cell to make opines: funny amino acids that only Agro can use

Agrobacterium tumefasciens (Rhizobium radiobacter) T-DNA contains “oncogenic genes” that cause overproduction of auxin and cytokinin: cause transformed cells to form tumors Also have gene forcing cell to make opines: funny amino acids that only Agro can use: convert host into factory feeding Agro!

Agrobacterium tumefasciens (Rhizobium radiobacter) T-DNA contains “oncogenic genes” that cause overproduction of auxin and cytokinin: cause transformed cells to form tumors Also have gene forcing cell to make opines: funny amino acids that only Agro can use: convert host into factory feeding Agro! Plant mol biologists have “disarmed” the Ti plasmid by removing “oncogenic genes” (remember Ti plasmid is 206,000 bp!)

Agrobacterium tumefasciens (Rhizobium radiobacter) Plant mol biologists have “disarmed” the Ti plasmid by removing “oncogenic genes” (remember Ti plasmid is 206,000 bp!) Added genes for plant and bacterial selectable markers Origins that work in E. coli and in Agrobacterium Promoter and terminator that work in plants

Agrobacterium tumefasciens (Rhizobium radiobacter) 1.Clone your gene into an E. coli plasmid

Agrobacterium tumefasciens (Rhizobium radiobacter) 1.Clone your gene into an E. coli plasmid 2.Add plant promoters and terminators

Agrobacterium tumefasciens (Rhizobium radiobacter) 1.Clone your gene into an E. coli plasmid 2.Add plant promoters and terminators 3.Transfer cassette into a disarmed (AKA binary) Ti plasmid between left and right border and transform into E. coli

Agrobacterium tumefasciens (Rhizobium radiobacter) 1.Clone your gene into an E. coli plasmid 2.Add plant promoters and terminators 3.Transfer cassette into a disarmed (AKA binary) Ti plasmid between left and right border and transform into E. coli 4.Verify plasmid, then transform into Agrobacterium

Agrobacterium tumefasciens (Rhizobium radiobacter) 1.Clone your gene into an E. coli plasmid 2.Add plant promoters and terminators 3.Transfer cassette into a disarmed (AKA binary) Ti plasmid between left and right border and transform into E. coli 4.Verify plasmid, then transform into Agrobacterium 5.Infect plants with this Agrobacterium: will transfer T-DNA carrying your gene into new host

Agrobacterium tumefasciens (Rhizobium radiobacter) Infect plants with this Agrobacterium: will transfer T-DNA carrying your gene into new host Select transgenic plants containing your new gene

Lipid metabolism Unique aspects in plants Make fatty acids by same reactions, but in plastids with a prokaryotic fatty acid synthase 12 proteins, cf one multifunctional protein

Lipid metabolism Make fatty acids in plastids with a prokaryotic FAS 12 proteins, instead of one multifunctional protein Assemble some lipids in CP, others in ER Acetyl-CoA carboxylase is also prokaryotic = 4 subunits, except in grasses (profoxydim & other grass herbicides inhibit ACCase)

Lipid metabolism “16:3 plants” assemble lipids in cp using FA-ACP = prokaryotic pathway (“primitive”) “18:3 plants” export FA, assemble lipids in ER using FA-CoA = eukaryotic pathway (“advanced”) Substrates for most desaturases are lipids, not FA!

Lipid metabolism Chloroplasts have lots of galactolipids: sugar linked directly to diacylglycerol : saves PO 4 A) MGDG (Monogalactosyl diacylglycerol) 50% cp B) DGDG (Digalactosyl diacylglycerol) 28% cp C) SQDG ( Sulphoquinovosyldiacylglycerol) 16% cp

Lipid metabolism Chloroplasts have lots of galactolipids: sugar linked directly to diacylglycerol : saves PO 4 A) MGDG (Monogalactosyl diacylglycerol) 50% cp B) DGDG (Digalactosyl diacylglycerol) 28% cp C) SQDG ( Sulphoquinovosyldiacylglycerol) 16% cp Very unsaturated! Makes membranes very fluid

Lipid metabolism Oleosomes: oil-storing organelles with only outer leaflet Put oils between the leaflets as they are made Add oleosin proteins to outside: curve the membrane Oils often have unusual fatty acids

Lipid metabolism Biological roles Plasma membrane lipids help survive freezing Unacclimated cells vesiculate as they lose water & pop when it returns Acclimated cells shrivel & reswell

Lipid metabolism Biological roles Plasma membrane lipids help survive freezing Mito lipid composition may also influence chilling sensitivity CS plants (eg bananas) are damaged at 10˚ C Mito show defects at <10˚ C not seen in other plants

Lipid metabolism CS plants (eg bananas) are damaged at 10˚ C Mito show defects at <10˚ C not seen in other plants Membrane lipids show phase changes at these T

Lipid metabolism CS plants (eg bananas) are damaged at 10˚ C Mito show defects at <10˚ C not seen in other plants Membrane lipids show phase changes at these T Blamed on saturated PG

Lipid metabolism Biological (& commercial) roles Plasma membrane lipids help survive freezing Mito lipid composition influences chilling sensitivity Mito show defects at <10˚ C not seen in other plants unsaturated FA did not fix CS, but saturated FA made it worse: reason for GM desaturases

Lipid metabolism Other commercial aspects Yield and quality (especially unsaturation) of seed oil is very important:12 million tons/year Want more double bonds, especially w-3, for health Want less double bonds for shelf life and taste Each double bond increases p(oxidation) 40x Have GM oils with more & less double bonds

Lipid metabolism Other commercial aspects Yield and quality of seed oil is very important:12 million tons/yr Also have markets for many specialized oils

Lipid metabolism Other commercial aspects Yield and quality of seed oil is very important Also have markets for many specialized oils Have genetically-engineered many crops to alter seed oils or produce specific fats

Lipid metabolism Biofuels are now very fashionable Biodiesel = fatty acid methyl esters Trans-esterify oils to make them volatile