Presentation is loading. Please wait.

Presentation is loading. Please wait.

CHAPTER SIX Nucleic acid hybridization: principles and applications 생물정보학협동과정 강민호.

Published byAlexandra Pitts Modified over 8 years ago

Similar presentations

Presentation on theme: "CHAPTER SIX Nucleic acid hybridization: principles and applications 생물정보학협동과정 강민호."— Presentation transcript:

1 CHAPTER SIX Nucleic acid hybridization: principles and applications 생물정보학협동과정 강민호

2 Nucleic Acid Hybridization Nucleic acid hybridization is a fundamental tool in molecular genetics which takes advantage of the ability of individual single-stranded nucleic acid molecules to form double stranded molecules (that is, to hybridize to each other)

3 - A labeled nucleic acid - a probe - to identify related DNA or RNA molecules - Complex mixture of unlabeled nucleic acid molecules- the target -Base complementarity with a high degree of similarity between the probe and the target. Standard nucleic acid hybridization assays

4 Types of probes

5 Probes DNA labelling –5’ –3’ –Uniform labeling Nick translation Random primer PCR-mediated labeling RNA labelling –In vitro transcription of a cloned DNA insert Different probes –Radioactive labeling or isotopic labeling –Nonradioactive labeling or nonisotopic labeling

6 Kinase end-labeling of oligonucleotides

7 Fill-in end labeling

8 Nick translation

9 Random primed labeling

10 Riboprobes

11 Characteristics of radioisotopes commonly used for labeling DNA and RNA probes RadioisotopeHalf-lifeDecay-typeEnergy of emission 3 H12.4 years  - 0.019 MeV 32 P14.3 days  - 1.710 MeV 33 P25.5 days  - 0.248 MeV 35 S87.4 days  - 0.167 MeV

12 Nonisotopic labeling and detection The use of nonradioactive labels has several advantages: –safety –higher stability of a probe –efficiency of the labeling reaction –detection in situ –less time taken to detect signal Major types –Direct nonisotopic labeling ( ex. nt labeled with a fluorophore ) –Indirect nonisotopic labeling ( ex. biotin.-streptavidin system )

13 Structure of fluorophores Fluorescence microscopy Common Fluorophores

14 Structure of digoxigenin-modified and biotin-modified nucleotides

15 Indirect nonisotopic labeling

16 Nucleic acid hybridization- formation of heteroduplexes

17 Denaturation of DNA results in an increase of optical density

18 Factors affecting Tm of nucleic acid hybrids Destabilizing agents ( ex. formamide, urea ) Ionic strenght Base composition ( G/C%, repetitive DNA) Mismatched base pairs Duplex lenght Different equations for calculating Tm for: DNA-DNA hybrids DNA-RNA hybrids RNA-RNA hybrids Oligonucleotide probes

19 Stringency High temperatureLow salt concentrationHigh denaturant concentration High strigency Low strigency Low temperature Sequence G/C content Sequence lenght Tm Low denaturant concentration High salt concentration Perfect match complementary sequences Perfect match non-complementary sequences

20 The identification of specific sequences in a complex mixture.

21 Filter hybridization techniques Filter hybridization methods Bacteriophage blotting Benton-Davis Bacterial colony blotting Grunstein-Hogness Slot/Dot blotting Northern analysis Southern analysis

22 Filters or Membranes Nitrocellulose Nylon Positive charged nylon (hybond) PVDF ( hydrophobic polyvinylidene difloride ) Different properties: –Binding capacity (mg nucleic acids/cm 2 ) –Tensile strenght –Mode of nucleic acid attachment –Lower size limit for efficient nucleic acid retention

23 Dot blot or slot blot

24 Principles of Southern blot

25 Northern Blot

26 Colony blot hybridization

27 In situ hybridization Chromosome in situ hybridization –Metaphase or protometaphase chromosomes are probed with labeled DNA. The DNA can be labeled with a fluorochrome (FISH). Tissue in situ hybridization –Sliced or whole mounted preparations can be probed with RNA probes to detect mRNA expression

28 Tissue In situ hybridization

29 Gridded clone hybridization

30 Construction of DNA and oligo microarrays

31 Gene expression profiling by hybridization

32 Summary I Hybridization is due to complementarity of DNA strands. DNA can be labeled various ways Isotopic and non isotopic Hybridization can detect identical or similar sequences.

33 Summary II A variety of techniques utilize hybridization of DNA or RNA probes –ASO –Southern Blot, RFLP, VNTRs, Mutation detection, deletion detection –Northern Blot, tissue specific expression –In situ hybridization Chromosome location and integrity Tissue specific expression

34 Summary III Colony hybridization can be used to identify specific clones. Once you have one clone you can find others that hybridize to it. Screening of gridded clones. One can identify genomic clones homologous to a cDNA or identify cDNA expressed in a cell line. Microarrays can be used in many ways to analyze gene expression in various cell types, in response to various stimuli.

Download ppt "CHAPTER SIX Nucleic acid hybridization: principles and applications 생물정보학협동과정 강민호."

Similar presentations

DNA strands can be separated under conditions which break H-bonds

DNA strands can be separated under conditions which break H-bonds
Recombinant DNA Technology

Recombinant DNA Technology
Online Counseling Resource YCMOU ELearning Drive… School of Architecture, Science and Technology Yashwantrao Chavan Maharashtra Open University, Nashik.

Online Counseling Resource YCMOU ELearning Drive… School of Architecture, Science and Technology Yashwantrao Chavan Maharashtra Open University, Nashik.
Nucleic Acid Hybridization Nucleic acid hybridization is a fundamental tool in molecular genetics which takes advantage of the ability of individual single-stranded.

Nucleic Acid Hybridization Nucleic acid hybridization is a fundamental tool in molecular genetics which takes advantage of the ability of individual single-stranded.
Chapter Six Nucleic Acid Hybridization: Principles & Applications 1.Preparation of nucleic acid probes: - DNA: from cell-based cloning or by PCR. Probe.

Chapter Six Nucleic Acid Hybridization: Principles & Applications 1.Preparation of nucleic acid probes: - DNA: from cell-based cloning or by PCR. Probe.
Hybridization of Nucleic Acids RNA DNA1DNA2 Probe Southern hybridization Northern hybridization Juang RH (2004) BCbasics.

Hybridization of Nucleic Acids RNA DNA1DNA2 Probe Southern hybridization Northern hybridization Juang RH (2004) BCbasics.
Nucleic Acid Hybridization Nucleic acids Complementary bases Hybridization Complementary strands from any sources Reversible reaction DNA/DNA or DNA/RNA.

Nucleic Acid Hybridization Nucleic acids Complementary bases Hybridization Complementary strands from any sources Reversible reaction DNA/DNA or DNA/RNA.
Molecular & Genomic Surgery Eric M. Wilson 1/5/10.

Molecular & Genomic Surgery Eric M. Wilson 1/5/10.
Гените са ДНК Част 1. 2 1.1 Introduction Figure 1.2.

Гените са ДНК Част Introduction Figure 1.2.
Gene Cloning, Expression, and Mutagenesis Type keywords: Molecular Cell Biology or DNA cloning and genomics.

Gene Cloning, Expression, and Mutagenesis Type keywords: Molecular Cell Biology or DNA cloning and genomics.
Additional Powerful Molecular Techniques Synthesis of cDNA (complimentary DNA) Polymerase Chain Reaction (PCR) Microarray analysis Link to Gene Therapy.

Additional Powerful Molecular Techniques Synthesis of cDNA (complimentary DNA) Polymerase Chain Reaction (PCR) Microarray analysis Link to Gene Therapy.
1 Library Screening, Characterization, and Amplification Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis.

1 Library Screening, Characterization, and Amplification Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis.
In situ Hybridization (ISH)

In situ Hybridization (ISH)
Basics of hybridization. What is hybridization? n Complementary base pairing of two single strands of nucleic acid  double strand product u DNA/DNA u.

Basics of hybridization. What is hybridization? n Complementary base pairing of two single strands of nucleic acid  double strand product u DNA/DNA u.
1 Characterization, Amplification, Expression Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis of DNA.

1 Characterization, Amplification, Expression Screening of libraries Amplification of DNA (PCR) Analysis of DNA (Sequencing) Chemical Synthesis of DNA.
General Microbiology (Micr300) Lecture 11 Biotechnology (Text Chapters: 10.15-10.17; 31.1-31.10)

General Microbiology (Micr300) Lecture 11 Biotechnology (Text Chapters: ; )
and analysis of gene transcription

and analysis of gene transcription
with an emphasis on DNA microarrays

with an emphasis on DNA microarrays
#Initial Phenotype of Mutant Complementation TestBeta-Gal AssayProbable Mutation 1RedWhiteBlue 2RedWhite 3RedNo growthWhite 4Red White 5Red White 6Red.

#Initial Phenotype of Mutant Complementation TestBeta-Gal AssayProbable Mutation 1RedWhiteBlue 2RedWhite 3RedNo growthWhite 4Red White 5Red White 6Red.
TOPICS IN (NANO) BIOTECHNOLOGY Lecture 7 5th May, 2006 PhD Course.

TOPICS IN (NANO) BIOTECHNOLOGY Lecture 7 5th May, 2006 PhD Course.

Similar presentations

Ads by Google