Presentation is loading. Please wait.

Presentation is loading. Please wait.

Chapter 20 Notes: DNA Technology. Understanding & Manipulating Genomes 1995: sequencing of the first complete genome (bacteria) 2003: sequencing of the.

Published byLee Fowler Modified over 8 years ago

Similar presentations

Presentation on theme: "Chapter 20 Notes: DNA Technology. Understanding & Manipulating Genomes 1995: sequencing of the first complete genome (bacteria) 2003: sequencing of the."— Presentation transcript:

1 Chapter 20 Notes: DNA Technology

2 Understanding & Manipulating Genomes 1995: sequencing of the first complete genome (bacteria) 2003: sequencing of the Human Genome mostly completed These accomplishments depended on new technology: –Recombinant DNA: DNA from 2 sources (often 2 species) are combined in vitro into the same DNA molecule Called Genetic engineering: direct manipulation of genes for practical purposes

3  DNA technology has launched a revolution in the area of:  BIOTECHNOLOGY: the use of living organisms or their components to do practical tasks -microorganisms to make wine/cheese -selective breeding of livestock -production of antibiotics -agriculture -criminal law

4 **Practical goal of biotech = improvement of human health and food production

5 Ch 20 looks at: 1.Main techniques for manipulating DNA 2.How genomes are analyzed & compared at the DNA level 3.Practical applications of DNA technology (including social & ethical issues)

6 “Toolkit” for DNA technology involves: -DNA vectors -host organisms - restriction enzymes

7 VECTORS = carriers for moving DNA from test tubes back into cells -bacterial plasmids (small, circular DNA molecules that replicate within bacterial cells) -viruses

8 HOST ORGANISMS: bacteria are commonly used as hosts in genetic engineering because: 1) DNA can easily be isolated from & reintroduced into bacterial cells; 2) bacterial cultures grow quickly, rapidly replicating any foreign genes they carry.

9 RESTRICTION ENZYMES = enzymes that recognize and cut short, specific nucleotide sequences (called restriction sites) -in nature, these enzymes protect the bacterial cell from other organisms by cutting up their foreign DNA

10 Restriction Enzymes (cont.)…  most restriction sequences are symmetrical in that the same sequence of 4-8 nucleotides is found on both strands, but run in opposite directions  restriction enzymes usually cut phosphodiester bonds of both strands in a staggered manner producing single stranded “sticky ends”

11

12 Restriction Enzymes (cont.)…  “sticky ends” of restriction fragments are used in the lab to join DNA pieces from different sources (complementary base pairing) *  RECOMBINANT DNA  unions of different DNA sources can be made permanent by adding DNA ligase enzyme (form covalent bonds between bases)

13

Download ppt "Chapter 20 Notes: DNA Technology. Understanding & Manipulating Genomes 1995: sequencing of the first complete genome (bacteria) 2003: sequencing of the."

Similar presentations

DNA Technology & Genomics

DNA Technology & Genomics
Chapter 20 DNA Technology & Genomics. Slide 2 of 14 Biotechnology Terms Biotechnology Process of manipulating organisms or their components to make useful.

Chapter 20 DNA Technology & Genomics. Slide 2 of 14 Biotechnology Terms Biotechnology Process of manipulating organisms or their components to make useful.
Changing the living world

Changing the living world
LEQ: HOW DO WE SPLICE NEW GENES INTO DNA? 12.1 to 12.7 and 12.18.

LEQ: HOW DO WE SPLICE NEW GENES INTO DNA? 12.1 to 12.7 and
Bacterial Transformation

Bacterial Transformation
Genetic engineering Recombinant DNA technology. Questions: Name 3 things you know about bacteria. What are some characteristics that make bacteria a good.

Genetic engineering Recombinant DNA technology. Questions: Name 3 things you know about bacteria. What are some characteristics that make bacteria a good.
Gene Cloning Techniques for gene cloning enable scientists to prepare multiple identical copies of gene-sized pieces of DNA. Most methods for cloning pieces.

Gene Cloning Techniques for gene cloning enable scientists to prepare multiple identical copies of gene-sized pieces of DNA. Most methods for cloning pieces.
RECOMBINANT DNA TECHNIQUE

RECOMBINANT DNA TECHNIQUE
 DNA – Double Helix Structure  Each spiral strand is composed of a sugar phosphate backbone and attached bases  4 Bases: Adenine (A), Guanine(G), Cytosine.

 DNA – Double Helix Structure  Each spiral strand is composed of a sugar phosphate backbone and attached bases  4 Bases: Adenine (A), Guanine(G), Cytosine.
Definitions: 1. Genetic engineering- remaking genes for practical purposes 2. Recombinant DNA- DNA made from two or more different organisms 3. Restriction.

Definitions: 1. Genetic engineering- remaking genes for practical purposes 2. Recombinant DNA- DNA made from two or more different organisms 3. Restriction.
GENETIC ENGINEERING (RECOMBINANT DNA TECHNOLOGY)

GENETIC ENGINEERING (RECOMBINANT DNA TECHNOLOGY)
Genetic Engineering Do you want a footer?.

Genetic Engineering Do you want a footer?.
Introduction to Biotech Notes MANIPULATING and ANALYZING DNA.

Introduction to Biotech Notes MANIPULATING and ANALYZING DNA.
Biotechnology The use of biological processes, organisms, or systems to manufacture products intended to improve the quality of human life.

Biotechnology The use of biological processes, organisms, or systems to manufacture products intended to improve the quality of human life.
Objective 2: TSWBAT describe the basic process of genetic engineering and the applications of it.

Objective 2: TSWBAT describe the basic process of genetic engineering and the applications of it.
CHAPTER 20 BIOTECHNOLOGY: PART I. BIOTECHNOLOGY Biotechnology – the manipulation of organisms or their components to make useful products Biotechnology.

CHAPTER 20 BIOTECHNOLOGY: PART I. BIOTECHNOLOGY Biotechnology – the manipulation of organisms or their components to make useful products Biotechnology.
Chapter 20~ DNA Technology & Genomics

Chapter 20~ DNA Technology & Genomics
DNA Technology n Now it gets real….. O.J. Simpson capital murder case,1/95-9/95 Odds of blood on socks in bedroom not being N. Brown-Simpson’s: 8.5 billion.

DNA Technology n Now it gets real….. O.J. Simpson capital murder case,1/95-9/95 Odds of blood on socks in bedroom not being N. Brown-Simpson’s: 8.5 billion.
Chapter 20~DNA Technology & Genomics. Who am I? Recombinant DNA n Def: DNA in which genes from 2 different sources are linked n Genetic engineering:

Chapter 20~DNA Technology & Genomics. Who am I? Recombinant DNA n Def: DNA in which genes from 2 different sources are linked n Genetic engineering:
DNA Technology Ch. 20 Figure 20.1 An overview of how bacterial plasmids are used to clone genes.

DNA Technology Ch. 20 Figure 20.1 An overview of how bacterial plasmids are used to clone genes.

Similar presentations

Ads by Google