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Biotechnology and Genomics Chapter 17 & 18 DNA Manipulation • Restriction endonucleases revolutionized molecular biology • Enzymes that cleave DNA at specific sites – Used by bacteria against viruses • Restriction enzymes significant – Allow a form of physical mapping that was previously impossible – Allow the creation of recombinant DNA molecules (from two different sources) 2 Recombinant DNA • Recombinant DNA (rDNA) contains DNA from two or more different sources. • Restriction enzymes cleave the vector DNA and the source DNA at a specific sequence. • Restriction enzymes • Used in manipulating DNA – Recognize specific DNA sequences – Cleave at specific site within sequence – Can lead to “sticky ends” that can be joined to allow a portion of the source DNA to be inserted into the vector DNA. 4 5 • DNA ligase - Joins the two fragments forming a stable recombinant DNA molecule. • After recombinant DNA enters the host cell, it may be copied. 6 Molecular Cloning • Clone – genetically identical copy • Occurs naturally in new plant shoots, bacterial colonies and identical human twins. • Gene cloning – isolation of a specific DNA sequence, producing identical copies of a gene. • The most flexible and common host for cloning is E. coli – Vector – carries DNA in host and can replicate in the host – Each host–vector system has particular uses 7 Vectors • A vector plasmid (a small accessory ring of DNA in bacteria) or virus is necessary to insert foreign DNA into a host cell. • Plasmids – Small, circular chromosomes – Used for cloning small pieces of DNA Bacterial cells take up recombinant plasmids and clone the new DNA. 8 9 DNA Libraries • A collection of DNAs in a vector that taken together represent the complex mixture of DNA • Genomic library – representation of the entire genome in a vector – Genome is randomly fragmented – Inserted into a vector – Introduced into host cells 10 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Plasmid Library DNA fragments from source DNA DN A inserted into plasmid vector Transformation Each cell contains a single fragment. All cells together are the library. 11 DNA Analysis • Restriction maps – Molecular biologists need maps to analyze and compare cloned DNAs – Initially, created by enzyme digestion, separation by electrophoresis, and analysis of resulting patterns – Many are now generated by computer searches for cleavage sites 12 Gel Electrophoresis • Separate DNA fragments by size (restriction enzymes) • Gel usually made of agarose • Submersed in buffer that can carry current • Subjected to an electrical field • Negatively-charged DNA migrates towards the positive pole • Larger fragments move slower, smaller move faster • DNA is visualized using fluorescent dyes • Results in a pattern unique to the individual (Genetic fingerprint) 13 14 15 • DNA fingerprinting – Identification technique used to detect differences in the DNA of individuals – Population is polymorphic for these markers – Using several probes, probability of identity can be calculated or identity can be ruled out – First used in a U.S. criminal trial in 1987 • Tommie Lee Andrews was found guilty of rape – Also used to identify remains 16 • Southern blotting – Sample DNA is digested by restriction enzymes and separated by gel electrophoresis – Double-stranded DNA denatured into singlestrands – Gel “blotted” with filter paper to transfer DNA – Filter is incubated with a labeled probe consisting of purified, single-stranded DNA corresponding to a specific gene 17 18 19 20 DNA Analysis 21 • DNA sequencing – Determination of actual base sequence of DNA – Basic idea is nested fragments – Each begin with the same sequence and end in a specific base – By starting with the shortest fragment, one can then read the sequence by moving up the ladder 22 • Polymerase chain reaction (PCR) – Developed by Kary Mullis • Awarded Nobel Prize – Produces many copies of a single gene or piece of DNA. Requires DNA polymerase and a supply of nucleotides for the new DNA strand. – Each PCR cycle involves three steps: 1.Denaturation (high temperature) 2.Annealing of primers (low temperature) 3.DNA synthesis (intermediate temperature) 23 After 20 cycles, a single fragment produces over one million (220) copies! 24 25 • Applications of PCR – Allows the investigation of minute samples of DNA – Forensics – drop of blood, cells at base of a hair – Detection of genetic defects in embryos by analyzing a single cell – Analysis of mitochondrial DNA from early human species 26 Genetic Engineering • Has generated excitement and controversy • Expression vectors contain the sequences necessary to express inserted DNA in a specific cell type • Transgenic organisms have had a foreign gene inserted in them. • Transgenic animals contain genes that have been inserted without the use of 27 conventional breeding Medical Applications • Transgenic bacteria - Medically important proteins can be produced in bacteria – Human insulin – Interferon – Hepatitis B vaccine – Human growth hormone – Problem has been purification of desired proteins from other bacterial proteins – Bacteria has been added to degrade waste and help mine metals. 28 Genetically engineered mouse with human growth hormone 29 • Gene therapy – Adding a functional copy of a gene to correct a hereditary disorder – Severe combined immunodeficiency disease (SCID) illustrates both the potential and the problems • On the positive side, 15 children treated successfully are still alive • On the negative side, three other children treated have developed leukemia (due to therapy) 30 Ex Vivo Gene Therapy • The ex vivo method withdraws tissues from the patient. Bone marrow stem cells are withdrawn from the body, a retrovirus is used to insert a normal gene into them, and the stem cells are returned to the body. • This method works for (SCIDs) and may work for familial hypercholesterlemia where liver cells lack a receptor for removing blood cholesterol. 31 In Vivo Gene Therapy • Cystic fibrosis patients lack a gene that codes for a membrane carrier of chloride ions; researchers try to deliver the gene by nose sprays. • Many researchers are trying to cure cancer by inserting genes to make healthy cells tolerant of chemotherapy or use gene p53 to bring about apoptosis of cancer cells. 32 Agricultural Applications • Transgenic plants - Foreign genes are added to protoplasts (lack a cell wall) using electric current. • Foreign genes in cotton, corn, and potatoes have given them pest resistance; soybeans are made resistence for no till farming. • Transgenic plants produce human hormones, clotting factors and antibodies 33 in their seeds. 34 35 • Herbicide resistance – Broadleaf plants have been engineered to be resistant to the herbicide glyphosate – Benefits • Crop resistant to glyphosate would not have to be weeded • Single herbicide instead of many types • Glyphosate breaks down in environment – In the United States, 90% of soy currently grown is GM soy 36 • Golden rice – Rice that has been genetically modified to produce b-carotene (provitamin A) – Converted in the body to vitamin A – Could not have been done by conventional breeding as no rice known produces these enzymes. – Available free with no commercial entanglements 37 38 • Adoption of genetically modified (GM) crops has been resisted in some areas because of questions – Crop safety for human consumption – Movement of genes into wild relatives • No evidence so far but it is not impossible 39 • Biopharming – Transgenic plants are used to produce pharmaceuticals – 1990 – Human serum albumin produced in genetically engineered tobacco and potato plants – In development • Recombinant subunit vaccines against Norwalk and rabies viruses • Recombinant monoclonal antibodies against tooth decay-causing bacteria 40 Transgenic animal technology • Has not been as successful as that in plants • Main use thus far has been engineering animals to produce pharmaceuticals in milk (also biopharming) • Can be inserted into eggs by hand or vortex mixing. • Gene farming uses transgenic farm animals to produce pharmaceuticals in milk. Plans to use animals to produce drugs for treatment of cystic fibrosis, cancer, etc. 41 Human Genome The Human Genome Project has two goals: • to know the sequence of bases on all the human chromosomes • to construct a map of genes on all the human chromosomes. • This task has been completed and researchers know the sequence of three billion base pairs after 15 years of research. • The two agencies that completed the task are The International Human Genome Sequencing Consortium and Celera Genomics, a private company. • However, knowledge of the sequence merely leads to additional work to determine how it acts. DNA sequences are similar among organisms and the differences may be due to regulation of genes. The Human Genome Project found fewer genes than expected -Initial estimate was 100,000 genes -Number now appears to be about 25,000 -However, the complexity of an organism is not necessarily related to its gene number Genomics Bioinformatics - Use of computer programs to search for genes, and to assemble and compare genomes Each cell in our bodies has about 6 feet of DNA stuffed into it • However, less than one inch is devoted to genes! Genome Organization Genomes consist of two main regions • Coding DNA - Contains genes than encode proteins • Noncoding DNA - Regions that do not encode proteins 46 Comparative Genomics • Comparative genomics, the study of whole genome maps of organisms, has revealed similarities among them • Comparing genomes (entire DNA sequences) of different species provides a powerful new tool for exploring the evolutionary divergence among organisms • Genomes are instructions and a history of life 47 Applications of Genomics • The genomics revolution will have a lasting effect on how we think about living systems • The immediate impact of genomics is being seen in diagnostics - Identifying genetic abnormalities - Identifying victims by their remains - Distinguishing between naturally occurring and intentional outbreaks of infections 48 Applications of Genomics • Genomics has also helped in agriculture – Improvement in the yield and nutritional quality of rice – Corn resistant to drought stress • - Doubling of world grain production in last 50 years, with only a 1% cropland increase 49 • Genome science is also a source of ethical challenges and dilemmas - Gene patents - Should the sequence/use of genes be freely available or can it be patented? - Privacy concerns - Could one be discriminated against because their SNP profile indicates susceptibility to a disease? 50 • Stem cells – Cells that are capable of continued division, but can also give rise to differentiated cells – Degree of determination • Totipotent – cell that can give rise to any tissue in an organism (embryo and extraembryonic membranes) • Pluripotent – give rise to all cells in the adult organism’s body • Multipotent – give rise to limited number of cells • Unipotent – give rise to only a single cell type 51 • Embryonic stem cells (ES cells) – Form of pluripotent stem cells – Made from mammalian blastocysts – ES cells isolated from inner cell mass and grown in culture – In mice, have been shown to develop into any type of cell in the tissues of the adult • Cannot develop into extraembryonic membranes – 1998 – first human ES cells • Great promise and controversy 52 53 Nuclear reprogramming • Early experiments showed nuclei could be transplanted between cells – Cells do not appear to undergo any truly irreversible changes, such as loss of genes – More differentiated the cell type, the less successful the nucleus in directing development when transplanted • Nuclear reprogramming – nucleus from a differentiated cell undergoes epigenetic changes that must be reversed to allow the nucleus to direct development 54 • 1984 – sheep was cloned using the nucleus from a cell of an early embryo • 1996 – Dolly, the first clone generated from a fully differentiated animal cell – Used somatic cell nuclear transfer (SCNT) – Dolly matured into fertile adult – Established beyond all dispute that determination in animals is reversible 55 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Preparation Cell Fusion Mammary cell is extracted and grown in nutrient-deficient solution that arrests the cell cycle. Nucleus containing source DNA Egg cell is extracted. Development Embryo begins to develop in vitro. Mammary cell is inserted inside covering of egg cell. Cell Division Electric shock fuses cell membranes and triggers cell division. Nucleus is removed fro egg cell with a micropipette. Implantation Birth of Clone Growth to Adulthood Embryo is After a five-month pregnancy, a implanted into lamb genetically identical to the surrogate sheep from which the mammary mother . cell was extracted is born. Embryo 56 © APTV/AP Photo • Reproductive cloning – Uses SCNT to create animal genetically identical to another – Efficiency is quite low and other problems • Only 3–5% of adult nuclei transferred to donor eggs result in live births – Due to lack of genomic imprinting • Normal mammalian development depends on precise genomic imprinting • Organization of chromatin in adult and embryo very different 57 • Much work has been put into trying to find ways to reprogram adult cells to become pluripotent cells without the use of embryos • Different lines of inquiry showed that reprogramming of somatic nuclei was possible • 2006 – genes for 4 different transcription factors introduced into fibroblast cells in culture – Named induced pluripotent stem cells (iPS cells) – Appear to be similar to ES cells in terms of developmental potential, as well as gene expression pattern 58 Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. Oocyte Nuclear Transfer Somatic cells Somatic cells Fusion Blastocyst ES cells Defined factors Culture Pluripotent stem cells Somatic cells Germ cells Some adult stem cells 59 • Therapeutic cloning – Produce patient-specific lines of embryonic stem cells – Artificial embryo created using same process as Dolly (SCNT) – Its cells are used as embryonic stem cells for transfer to injured tissue – Body readily accepts these cells with no immune rejection – May be obsolete with development of iPS 60 cells Copyright © The McGraw-Hill Companies, Inc. Permission required for reproduction or display. The nucleus from a skin cell of a diabetic patient is removed. The skin cell nucleus is inserted into the enucleated human egg cell. Cell cleavage occurs as the embryo begins to develop in vitro. The embryo reaches the blastocyst stage. Inner cell mass Diabetic patient Early embryo ES cells Blastocyst Therapeutic cloning Embryonic stem cells (ES cells) are extracted and grown in culture. The stem cells are developed into healthy pancreatic islet cells needed by the patient. Healthy pancreatic islet cells The healthy tissue is injected or transplanted into the diabetic patient. Diabetic patient 61 Morphogenesis • Generation of ordered form and structure • Product of changes in cell structure and cell behavior • Animals regulate – – – – – The number, timing, and orientation of cell divisions Cell growth and expansion Changes in cell shape Cell migration (not used in plants) Cell death 62 • Apoptosis – Programmed cell death a part of development • Human embryos begin with webbed fingers, but webbing “dies” as part of development. – Necrosis – cells that die due to injury 63