Concepts and Methods in Developmental Biology

Similar documents
A Survey of Genetic Methods

Biology 4361 Developmental Biology Lecture 4. The Genetic Core of Development

Genetics - Problem Drill 19: Dissection of Gene Function: Mutational Analysis of Model Organisms

Exam 1 ID#: October 16, 2007

Experimental genetics - 2 Partha Roy

Exam 1 ID#: June 23, Multiple choice (one point each; indicate the best answer)

Exam 1 ID#: October 1, 2006

Student Learning Outcomes (SLOS) - Advanced Cell Biology

Genetics Faculty of Agriculture and Veterinary Medicine. Instructor: Dr. Jihad Abdallah Topic 16: Biotechnology

Lecture 17. Transgenics. Definition Overview Goals Production p , ,

Introducing new DNA into the genome requires cloning the donor sequence, delivery of the cloned DNA into the cell, and integration into the genome.

Prof. Fahd M. Nasr. Faculty of Sciences Lebanese University Beirut, Lebanon.

OmicsLink shrna Clones guaranteed knockdown even in difficult-to-transfect cells

Biotech Applications Nucleic acid therapeutics, Antibiotics, Transgenics. BIT 220 End of Chapter 22 (Snustad/Simmons)

KEY Reproductive cloning Therapeutic cloning

LIFE. How-to 2 Cloning and Epigenetics. More great student questions of the day. 1. Reproductive vs therapeutic cloning

Developmental Biology 3230 Exam 1 (Feb. 6) NAME

Concept 13.1 Recombinant DNA Can Be Made in the Laboratory

John Gurdon was testing the hypothesis of genomic equivalence or that when cells divide they retain a full genomic compliment.

Technical tips Session 4

Lecture 8: Transgenic Model Systems and RNAi

Chapter 19 Genetic Regulation of the Eukaryotic Genome. A. Bergeron AP Biology PCHS

Test Bank for Molecular Cell Biology 7th Edition by Lodish

Value Correct Answer Feedback. Student Response. A. Dicer enzyme. complex. C. the Dicer-RISC complex D. none of the above

Stem Cel s Key Words:

Control of Eukaryotic Gene Expression (Learning Objectives)

Chapter 1. from genomics to proteomics Ⅱ

Learning Objectives. Define RNA interference. Define basic terminology. Describe molecular mechanism. Define VSP and relevance

DB3230 Midterm 1 11/15/2013 Name:

RNA folding and its importance. Mitesh Shrestha

It s All in the Hands Genetic Engineering

The first experiments

TRANSGENIC ANIMALS. -transient transfection of cells -stable transfection of cells. - Two methods to produce transgenic animals:

TRANSGENIC ANIMALS. transient. stable. - Two methods to produce transgenic animals:

PhysicsAndMathsTutor.com. Question Number. Answer Additional guidance Mark. 1(a) 1. reference to stem cells being {totipotent / pluripotent} ;

Transgenesis. Stable integration of foreign DNA into host genome Foreign DNA is passed to progeny germline transmission

Chapter 5 Genetic Analysis in Cell Biology. (textbook: Molecular Cell Biology 6 ed, Lodish section: )

Cloning and Epigenetics. Developmental Readout. Foundations. Human issues. Stem cells. Cloning. Axon guidance.

Control of Eukaryotic Genes. AP Biology

Chapter 11: Applications of Biotechnology

Biotechnology and DNA Technology

CELL BIOLOGY - CLUTCH CH. 7 - GENE EXPRESSION.

GENE EXPRESSSION. Promoter sequence where RNA polymerase binds. Operator sequence that acts as a switch (yellow) OPERON

EUKARYOTIC GENE CONTROL

Name AP Biology Mrs. Laux Take home test #11 on Chapters 14, 15, and 17 DUE: MONDAY, DECEMBER 21, 2009

RNA Interference (RNAi) (see also mirna, sirna, micrna, shrna, etc.)

AP Biology Gene Expression/Biotechnology REVIEW

pdsipher and pdsipher -GFP shrna Vector User s Guide

RNA Structure and the Versatility of RNA. Mitesh Shrestha

Chapter 11. How Genes Are Controlled. Lectures by Edward J. Zalisko

2014 Pearson Education, Inc. CH 8: Recombinant DNA Technology

There are four major types of introns. Group I introns, found in some rrna genes, are self-splicing: they can catalyze their own removal.

Exam 3 4/25/07. Total of 7 questions, 100 points.

Cloning and Genetic Engineering

Biotechnology Unit 3: DNA to Proteins. From DNA to RNA

Biotechnology. Professor Andrea Garrison Biology 11 Illustrations 2010 Pearson Education, Inc., unless otherwise noted

Eukaryotic Regulation

RNAi minilecture and Using Genetics to Explore Complex Biological Processes

CH 8: Recombinant DNA Technology

TOOLS sirna and mirna. User guide

What is Biotechnology? 15.1 What is Biotechnology? Transgenic Biotechnology Transgenic Biotechnology. Biotechnology. Transgenic organism

RNAi HTS and Data Analysis

2. Outline the levels of DNA packing in the eukaryotic nucleus below next to the diagram provided.

ANAT 2341 Embryology Lecture 18 Stem Cells

Genetic Technologies

AQA Biology A-level Topic 8: The control of gene expression

MISSION shrna Library: Next Generation RNA Interference

Bart Williams, PhD Van Andel Research Center

Technology Overview. Figure 1. asirna structure

RNA genes. Functional non-coding RNAs (ncrna) Jan 31 st 2018.

2054, Chap. 14, page 1

Exam 1 ID#: June 29, 2009

Recombinant DNA Technology. The Role of Recombinant DNA Technology in Biotechnology. yeast. Biotechnology. Recombinant DNA technology.

Molecular Medicine. Stem cell therapy Gene therapy. Immunotherapy Other therapies Vaccines. Medical genomics

RNA Interference (RNAi) (see also sirna, micrna, shrna, etc.)

RNA Interference (RNAi) (see also sirna, micrna, shrna, etc.)

Applicazioni biotecnologiche

Control of Eukaryotic Genes

Division Ave. High School AP Biology

Lecture 15: Functional Genomics II

Human Molecular Genetics Assignment 3 (Week 3)

Control of Eukaryotic Genes. AP Biology

TRANSGENIC TECHNOLOGIES: Gene-targeting

Edexcel (B) Biology A-level

Lectures 28 and 29 applications of recombinant technology I. Manipulate gene of interest

4/26/2015. Cut DNA either: Cut DNA either:

Mouse Engineering Technology. Musculoskeletal Research Center 2016 Summer Educational Series David M. Ornitz Department of Developmental Biology

New Plant Breeding Technologies

Analysis of gene function

Genetic Engineering. Genetically Modified Organisms (GMO s)

Stem Cells & Neurological Disorders. Said Ismail Faculty of Medicine University of Jordan

B5 Growth and development. B5 Growth and development. Question How many different bases are found in DNA?

WORKING WITH THE FIGURES. 1. In Figure 8-3, why are the arrows for genes 1 and 2 pointing in opposite directions?

species- Mus musculus Engineering the mouse genome David Ornitz

CBA #4 Practice Exam Genetics. 1) (TEKS 5A) Which of the diagrams below shows the process of transcription:

Chapter 20 Recombinant DNA Technology. Copyright 2009 Pearson Education, Inc.

Stem Cell review/cloning Section. If false, correct only one of the underlined words to make the statement true.

Genetics and Genomics in Medicine Chapter 9 Questions

New microribbon production

12/31/16. I. Manipulating DNA (9.1) A. Scientists use several techniques to manipulate DNA. 1. DNA is a very large molecule

Transcription:

Biology 4361 Developmental Biology Concepts and Methods in Developmental Biology June 16, 2009

Conceptual and Methodological Tools Concepts Genomic equivalence Differential gene expression Differentiation/de-differentiation Technical Methods Cloning RNA localization techniques RT-PCR microarrays macroarrays in situ hybridization Transgenics microinjection chimeras embryonic stem cells Gene knockouts, etc. Antisense RNA RNA interference

Differentiation Overview Differentiation cells become structurally and functionally different Selective expression of certain genes = production of specific proteins Specific proteins = specialized cell Differentiation: one-way (i.e. normally, no de-differentiation) Detecting differentiation (or stages): differential gene expression mrna DNA transcription protein whole cell techniques

Concept: Genomic Equivalence Every cell in an organism has the same set of genes. If so, shouldn t any nucleus be able to direct the development of any other cell, even the zygote? Test: somatic nuclear transplantation (cloning) - use a somatic (i.e. differentiated) nucleus to direct development Technical challenges: - enucleation of a recipient egg - acquisition of competent donor nuclei - ability to transfer nuclei into enucleated oocytes

Method - Amphibian Cloning (activates egg)

Effect of Age in Nuclear Transplants Transplant nuclei from different aged donors. Rana pipiens Loss of ability of nuclei to support development = loss of blastomere potency

Serial Transplantation Clones made with differentiated nuclei died shortly after the blastula stage. However, if blastomeres from cloned blastulae were used as nuclear donors. and the process was repeated several times. clones could survive. Xenopus laevis Differentiated nuclei still had pluripotent potential but de-differentiation was necessary

Method - Mammalian Cloning Udder cell - differentiated

Mammalian Cloning - 2 Inner cell mass (ICM) forms embryo proper Trophoblast forms connections with placenta Mammalian cloning success in multiple species, however - inefficient (Dolly = 1/434 transfers) Problems: - large fetus - old chromosomes - disease susceptibility - premature aging

Concept: Differential Gene Expression Changes seen in blastomeres as they age = changes in the expression of genes, not in the content of the genome. Differential gene expression is the key to changing phenotype of the cell.

Concept: Differential Gene Expression Three postulates of differential gene expression: 1. Every nucleus contains the complete genome; DNAs of all differentiated cells are identical. 2. Unexpressed genes in differentiated cells are not destroyed or mutated, but retain the potential for being expressed. - during development, cells constantly change function - serial nuclear transplantation showed re-programming of differentiated cells 3. Only a small percentage of the genome is expressed in each cell. - polytene chromosomes illustrate expression patterns

Polytene Chromosomes (Drosophila) Illustrate genomic equivalence and differential gene transcription: - banding patterns same in different cell types (i.e. same chromosomes) - however, patterns of transcriptional activity are different

Chromosome Puffs Active Transcription Puffs represent active gene transcription Claus Pelling, Max-Planck Institute of Biology, Tübingen. control + actinomycin (prevents RNA synthesis) - changing patterns over time = regulation of transcriptional activity Timed sequence of Drosophila chromosome puffs; ~ 20 h Michael Ashburner, University of Cambridge

Method - Transgenic Cells and Organisms Transgenics move genes in (or out) of organisms Why?

Method - Chimera Formation Mammalian blastocyst inner cell mass - embryo proper trophoblast - embryonic contribution to the placenta insert gene into embryo using - transfection - microinjection - etc. NOTE - vector contains antibiotic resistance gene

- and some may integrate into the germ line (gamete progenitors) Method - Chimera Formation ES cells (with transgene and antibiotic resistance gene) NOTE growth medium contains antibiotic!

mouse (R) - transgenic for human growth hormone R. L. Brinster and R. E. Hammer

Method - Gene Knockouts Targeted gene insertion - similar to chimeric method, but.. - selectively replaces functional genes with non-functional genes target gene: bone morphogenic protein 7 (BMP7) mutation: insert a gene for neomycin resistance into the BMP7 gene regions of homology - neo r = neomycin resistance

The presence of the antibioticresistance gene allows selection of only successfully incorporated knockout genes

Method - Antisense RNA mrna single stranded message = sense strand: 5 C-A-U-G3 complement (synthesized) = antisense strand: 3 G-U-A-C5 Insertion of antisense RNAs into the cell blocks gene expression: - translational blockage (synthetic antisense RNAs) - transcriptional blockage - postulated function of natural antisense RNAs

Methods Method - Antisense RNA Synthesis and insertion of antisense RNA - binds to native mrna - double stranded RNA subject to enzymatic destruction (Dicer) Morpholino antisense oligomers - morpholino molecules used in strand construction - morpholino oligomers do not degrade; effective over several cell generations morpholino Note - naturally-occurring antisense RNAs also exist: - paternal gene for IGF2r receptor contains antisense sequence - blocks synthesis of IGF2r

Method - RNA-Interference RNA interference (RNAi) - double-stranded RNAs inserted (short interfering RNA (sirna) - leads to the degradation of native mrna - RNAi is common in plants, animals, fungi - probably evolved as a defense against retroviruses = dsrnas

Method - RNA-Interference Dicer enzyme complex binds to dsrna - cleaves into short interfering RNA (sirna) Note - when dsrna is from endogenous source = microrna (mirna) RISC (RNA induced silencing complex) - argonaut component of Dicer complex catalyzes mrna degradation

RNAi mechanisms triggers: RNAi Knockdown RNAi-inhibited transcription: knockdown experiments - blocks transcription of specific genes - lack of gene = lack of protein = lack of function - advantage: effect can be seen at certain time in certain tissue - like knockouts, but not as complete - sirnas specific for particular sequence - mirnas less specificity mirna stem-loop sirna dsrna, probably from RNA viruses aka short hairpinrna (shrna) microrna (mirna) - genetically coded sequences; - non-coding; - control some translation during portions of development - extensive post-transcriptional modification

2024 © businessdocbox.com Privacy Policy | Terms of Service | Feedback