SlideShare a Scribd company logo

PCR experiment practice for undergraduate student

Download as PPTX, PDF
Nguyen Nhung
Nguyen Nhung

~^^ If you wonder when you first do PCR, how it looks in real experiment. Enjoy!

Education
1 of 22
Class of Modern Life Science Laboratory - May, 2014 - T.A Hong Nhung Nguyen & 서보경 Experiment 10 Polymerase Chain Reaction (PCR)
Contents ①Introduction ②Materials and Methods ③Result and Discussion ④Trouble shooting  Purpose of today’s experiment  What is PCR?
Purpose of today’s experiment① Introduction www.expeditions.udel.edu Our previous experiments (A) (B) (C) Purpose: Amplify a “DNA fragment of interest” in genomic DNA, total cDNA, plasmid.
Dr. Kary Mullis, the inventor of PCR, was awarded the 1993 Nobel Prize in Chemistry. PCR invention and definition① Introduction  PCR is a technique which is used to amplify a specific region of DNA, in order to produce enough DNA to be adequately tested.  A special DNA polymerase (Taq) is used to make many copies of a short DNA fragment (100-10,000 bp) defined by primers.
81,267,844 bp 81,572,676 bp start end ATG10 is located at 5q14.1, size: 304,833 bases Autophagy Related Gene 10 (ATG10) in Chromosome 5 ATG10 …. PCR to amplify a DNA fragment of interest (861 bp) ① Introduction
81,267,844 bp 81,572,676 bp start end ATG10 is located at 5q14.1, size: 304,833 bases ATG10 …. PCR to amplify a DNA fragment of interest (861 bp) Forward and Reverse primers location in genomic DNA
for PCR (to amplify a “DNA fragment of interest)Materials and Methods 1. DNA template 2. Primer (10 pmol) 3. Taq DNA Polymerase 4. dNTPs mixture (10 mM) 5. Taq Buffer 10X and 25 mM MgCl2 mixed 6. 5X band doctor (Purchased from Solgent) use only when template DNA is genomic DNA PCR machine 1. DNA (genomic DNA isolated from human or Arabidopsis) Stock concentration: 500 ng/ul 2. cDNA (complementary DNA) synthesize from RNA after Reverse Transcriptase (RT) 3. Plasmid DNA Stock concentration: 50 ug/ul Mixture of Forward and Reverse primer (Listed as detail in your protocol) Stock 5U/ul, speed of synthesize: 1 minute/1 kb
Mixture Add DNA template to each sample Experimental design and prepare the mixture PCR machine programming PCR machine Thermocycles
Methods Programming Polymerase Chain Reaction Gene Sequence (5’-->3’ direction) Template DNA Tm Expected size(kb) gDNA ATG10-F GAA CAT CCA ATA CTT GGG CAA C MCF-7 gDNA 0.86 ATG10-R AGG GAC ATT TCG TTC ATC CTG 53 53 ? Extension time
PCR in test tubes Melting 94 oC Temperature 100 0 50 Time 5’3’ 3’5’
PCRMelting 94 oC Temperature 100 0 50 Time 3’5’ 5’3’ Heat
PCRMelting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 3’5’ 5’3’ 5’ 5’ Melting 94 oC
PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ Heat Heat 5’ 5’ 5’
PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’
PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’ Heat Heat
PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’
Fragments of defined length PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’
 Why PCR product using cDNA as template sometimes smaller in size? Result PCR using ATG10 F/R specific primer with different templates Where primer should be pick to check mRNA level? 861 bp 207 bp
Gene Sequence (5’-->3’ direction) Template DNA Annealing Tm Expected size(kb) gDNA ATG10-F GAA CAT CCA ATA CTT GGG CAA C MCF-7 gDNA 0.86 ATG10-R AGG GAC ATT TCG TTC ATC CTG 53 53 http://genome.ucsc.edu Isoform 1 Isoform 2 Isoform 3 861 bp 207 bp
Expected size Common troubles in PCRTroubleshooting Contamination?? Expected size No band?? ??
Summary 1. PCR is a technique which is used to amplify a specific region of DNA, in order to produce enough DNA to be adequately tested. 2. PCR is very sensitive 3. PCR need to be well-design and perform in optimal condition Today: Amplify a “DNA fragment of interest” in genomic DNA, total cDNA, plasmid. 861 bp 207 bp
PCR experiment practice for undergraduate student

Recommended

Pcr
PcrPcr
Pcr
Yohannes Gemechu
 
M Sc Project
M Sc ProjectM Sc Project
M Sc Project
Centre for Biotechnology, Turku
 
Pcr protocol
Pcr protocolPcr protocol
Pcr protocol
Areeba Ali
 
Bacteria
BacteriaBacteria
Bacteria
barshingert
 
Chloroplast Bibo
Chloroplast BiboChloroplast Bibo
Chloroplast Bibo
Bibrita Bhar
 
Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...
Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...
Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...
Hala Issa
 
Bio 127 lec 5 Microbiology: Physiological Requirements of bacteria
Bio 127 lec 5 Microbiology: Physiological Requirements of bacteriaBio 127 lec 5 Microbiology: Physiological Requirements of bacteria
Bio 127 lec 5 Microbiology: Physiological Requirements of bacteria
Shaina Mavreen Villaroza
 
Reaction time ppt
Reaction time pptReaction time ppt
Reaction time ppt
Zinat Ashnagar
 

Recommended

Pcr
PcrPcr
Pcr
Yohannes Gemechu
 
M Sc Project
M Sc ProjectM Sc Project
M Sc Project
Centre for Biotechnology, Turku
 
Pcr protocol
Pcr protocolPcr protocol
Pcr protocol
Areeba Ali
 
Bacteria
BacteriaBacteria
Bacteria
barshingert
 
Chloroplast Bibo
Chloroplast BiboChloroplast Bibo
Chloroplast Bibo
Bibrita Bhar
 
Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...
Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...
Differential Detection of Entamoeba dispar and Entamoeba moshkovskii Using ne...
Hala Issa
 
Bio 127 lec 5 Microbiology: Physiological Requirements of bacteria
Bio 127 lec 5 Microbiology: Physiological Requirements of bacteriaBio 127 lec 5 Microbiology: Physiological Requirements of bacteria
Bio 127 lec 5 Microbiology: Physiological Requirements of bacteria
Shaina Mavreen Villaroza
 
Reaction time ppt
Reaction time pptReaction time ppt
Reaction time ppt
Zinat Ashnagar
 
Bacterial Physiology and genetics
Bacterial Physiology and geneticsBacterial Physiology and genetics
Bacterial Physiology and genetics
Ibo Barznji
 
Plasmid Isolation Lab Report
Plasmid Isolation Lab ReportPlasmid Isolation Lab Report
Plasmid Isolation Lab Report
Mahmud Nabi
 
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
JYOTI DEVENDRA
 
Mirna 2017
Mirna 2017Mirna 2017
Mirna 2017
lalvarezmex
 
Whole Transcriptome Amplfication from Single Cell
Whole Transcriptome Amplfication from Single CellWhole Transcriptome Amplfication from Single Cell
Whole Transcriptome Amplfication from Single Cell
QIAGEN
 
Micro rna
Micro rnaMicro rna
Micro rna
alishahsavan20
 
Molecular detection of food borne pathogens-presentation
Molecular detection of food borne pathogens-presentationMolecular detection of food borne pathogens-presentation
Molecular detection of food borne pathogens-presentation
Yakindra Timilsena, PhD
 
Agarose Gel
Agarose GelAgarose Gel
Agarose Gel
Jessica Ong
 
Polymerase chain reaction
Polymerase chain reactionPolymerase chain reaction
Polymerase chain reaction
Aisha Kalsoom
 
Jose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptx
Jose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptxJose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptx
Jose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptx
ricssacare
 
The Last Leaf, a short story by O. Henry
The Last Leaf, a short story by O. HenryThe Last Leaf, a short story by O. Henry
The Last Leaf, a short story by O. Henry
Eugene Lysak
 
Sectors of the Indian Economy - Class 10 Study Notes pdf
Sectors of the Indian Economy - Class 10 Study Notes pdfSectors of the Indian Economy - Class 10 Study Notes pdf
Sectors of the Indian Economy - Class 10 Study Notes pdf
Vivekanand Anglo Vedic Academy
 
How to Create Map Views in the Odoo 17 ERP
How to Create Map Views in the Odoo 17 ERPHow to Create Map Views in the Odoo 17 ERP
How to Create Map Views in the Odoo 17 ERP
Celine George
 
GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...
GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...
GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...
Nguyen Thanh Tu Collection
 
Salient features of Environment protection Act 1986.pptx
Salient features of Environment protection Act 1986.pptxSalient features of Environment protection Act 1986.pptx
Salient features of Environment protection Act 1986.pptx
akshayaramakrishnan21
 
B.ed spl. HI pdusu exam paper-2023-24.pdf
B.ed spl. HI pdusu exam paper-2023-24.pdfB.ed spl. HI pdusu exam paper-2023-24.pdf
B.ed spl. HI pdusu exam paper-2023-24.pdf
Special education needs
 
Sha'Carri Richardson Presentation 202345
Sha'Carri Richardson Presentation 202345Sha'Carri Richardson Presentation 202345
Sha'Carri Richardson Presentation 202345
beazzy04
 
Benefits and Challenges of Using Open Educational Resources
Benefits and Challenges of Using Open Educational ResourcesBenefits and Challenges of Using Open Educational Resources
Benefits and Challenges of Using Open Educational Resources
dimpy50
 
How to the fix Attribute Error in odoo 17
How to the fix Attribute Error in odoo 17How to the fix Attribute Error in odoo 17
How to the fix Attribute Error in odoo 17
Celine George
 
MARUTI SUZUKI- A Successful Joint Venture in India.pptx
MARUTI SUZUKI- A Successful Joint Venture in India.pptxMARUTI SUZUKI- A Successful Joint Venture in India.pptx
MARUTI SUZUKI- A Successful Joint Venture in India.pptx
bennyroshan06
 
slides CapTechTalks Webinar May 2024 Alexander Perry.pptx
slides CapTechTalks Webinar May 2024 Alexander Perry.pptxslides CapTechTalks Webinar May 2024 Alexander Perry.pptx
slides CapTechTalks Webinar May 2024 Alexander Perry.pptx
CapitolTechU
 
[GDSC YCCE] Build with AI Online Presentation
[GDSC YCCE] Build with AI Online Presentation[GDSC YCCE] Build with AI Online Presentation
[GDSC YCCE] Build with AI Online Presentation
GDSCYCCE
 

More Related Content

Viewers also liked

sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
JYOTI DEVENDRA
 
Whole Transcriptome Amplfication from Single Cell
Whole Transcriptome Amplfication from Single CellWhole Transcriptome Amplfication from Single Cell
Whole Transcriptome Amplfication from Single Cell
QIAGEN
 
Molecular detection of food borne pathogens-presentation
Molecular detection of food borne pathogens-presentationMolecular detection of food borne pathogens-presentation
Molecular detection of food borne pathogens-presentation
Yakindra Timilsena, PhD
 
Polymerase chain reaction
Polymerase chain reactionPolymerase chain reaction
Polymerase chain reaction
Aisha Kalsoom
 

Viewers also liked (9)

Bacterial Physiology and genetics
Bacterial Physiology and geneticsBacterial Physiology and genetics
Bacterial Physiology and genetics
 
Plasmid Isolation Lab Report
Plasmid Isolation Lab ReportPlasmid Isolation Lab Report
Plasmid Isolation Lab Report
 
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
sem4-cdna sythesis,pcr,designing primers for pcr, synthesis of genes, shotgun...
 
Mirna 2017
Mirna 2017Mirna 2017
Mirna 2017
 
Whole Transcriptome Amplfication from Single Cell
Whole Transcriptome Amplfication from Single CellWhole Transcriptome Amplfication from Single Cell
Whole Transcriptome Amplfication from Single Cell
 
Micro rna
Micro rnaMicro rna
Micro rna
 
Molecular detection of food borne pathogens-presentation
Molecular detection of food borne pathogens-presentationMolecular detection of food borne pathogens-presentation
Molecular detection of food borne pathogens-presentation
 
Agarose Gel
Agarose GelAgarose Gel
Agarose Gel
 
Polymerase chain reaction
Polymerase chain reactionPolymerase chain reaction
Polymerase chain reaction
 

Recently uploaded

The basics of sentences session 4pptx.pptx
The basics of sentences session 4pptx.pptxThe basics of sentences session 4pptx.pptx
The basics of sentences session 4pptx.pptx
heathfieldcps1
 
Basic Civil Engg Notes_Chapter-6_Environment Pollution & Engineering
Basic Civil Engg Notes_Chapter-6_Environment Pollution & EngineeringBasic Civil Engg Notes_Chapter-6_Environment Pollution & Engineering
Basic Civil Engg Notes_Chapter-6_Environment Pollution & Engineering
Denish Jangid
 

Recently uploaded (20)

Jose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptx
Jose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptxJose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptx
Jose-Rizal-and-Philippine-Nationalism-National-Symbol-2.pptx
 
The Last Leaf, a short story by O. Henry
The Last Leaf, a short story by O. HenryThe Last Leaf, a short story by O. Henry
The Last Leaf, a short story by O. Henry
 
Sectors of the Indian Economy - Class 10 Study Notes pdf
Sectors of the Indian Economy - Class 10 Study Notes pdfSectors of the Indian Economy - Class 10 Study Notes pdf
Sectors of the Indian Economy - Class 10 Study Notes pdf
 
How to Create Map Views in the Odoo 17 ERP
How to Create Map Views in the Odoo 17 ERPHow to Create Map Views in the Odoo 17 ERP
How to Create Map Views in the Odoo 17 ERP
 
GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...
GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...
GIÁO ÁN DẠY THÊM (KẾ HOẠCH BÀI BUỔI 2) - TIẾNG ANH 8 GLOBAL SUCCESS (2 CỘT) N...
 
Salient features of Environment protection Act 1986.pptx
Salient features of Environment protection Act 1986.pptxSalient features of Environment protection Act 1986.pptx
Salient features of Environment protection Act 1986.pptx
 
B.ed spl. HI pdusu exam paper-2023-24.pdf
B.ed spl. HI pdusu exam paper-2023-24.pdfB.ed spl. HI pdusu exam paper-2023-24.pdf
B.ed spl. HI pdusu exam paper-2023-24.pdf
 
Sha'Carri Richardson Presentation 202345
Sha'Carri Richardson Presentation 202345Sha'Carri Richardson Presentation 202345
Sha'Carri Richardson Presentation 202345
 
Benefits and Challenges of Using Open Educational Resources
Benefits and Challenges of Using Open Educational ResourcesBenefits and Challenges of Using Open Educational Resources
Benefits and Challenges of Using Open Educational Resources
 
How to the fix Attribute Error in odoo 17
How to the fix Attribute Error in odoo 17How to the fix Attribute Error in odoo 17
How to the fix Attribute Error in odoo 17
 
MARUTI SUZUKI- A Successful Joint Venture in India.pptx
MARUTI SUZUKI- A Successful Joint Venture in India.pptxMARUTI SUZUKI- A Successful Joint Venture in India.pptx
MARUTI SUZUKI- A Successful Joint Venture in India.pptx
 
slides CapTechTalks Webinar May 2024 Alexander Perry.pptx
slides CapTechTalks Webinar May 2024 Alexander Perry.pptxslides CapTechTalks Webinar May 2024 Alexander Perry.pptx
slides CapTechTalks Webinar May 2024 Alexander Perry.pptx
 
[GDSC YCCE] Build with AI Online Presentation
[GDSC YCCE] Build with AI Online Presentation[GDSC YCCE] Build with AI Online Presentation
[GDSC YCCE] Build with AI Online Presentation
 
An Overview of the Odoo 17 Discuss App.pptx
An Overview of the Odoo 17 Discuss App.pptxAn Overview of the Odoo 17 Discuss App.pptx
An Overview of the Odoo 17 Discuss App.pptx
 
How to Manage Notification Preferences in the Odoo 17
How to Manage Notification Preferences in the Odoo 17How to Manage Notification Preferences in the Odoo 17
How to Manage Notification Preferences in the Odoo 17
 
size separation d pharm 1st year pharmaceutics
size separation d pharm 1st year pharmaceuticssize separation d pharm 1st year pharmaceutics
size separation d pharm 1st year pharmaceutics
 
The basics of sentences session 4pptx.pptx
The basics of sentences session 4pptx.pptxThe basics of sentences session 4pptx.pptx
The basics of sentences session 4pptx.pptx
 
Phrasal Verbs.XXXXXXXXXXXXXXXXXXXXXXXXXX
Phrasal Verbs.XXXXXXXXXXXXXXXXXXXXXXXXXXPhrasal Verbs.XXXXXXXXXXXXXXXXXXXXXXXXXX
Phrasal Verbs.XXXXXXXXXXXXXXXXXXXXXXXXXX
 
The Art Pastor's Guide to Sabbath | Steve Thomason
The Art Pastor's Guide to Sabbath | Steve ThomasonThe Art Pastor's Guide to Sabbath | Steve Thomason
The Art Pastor's Guide to Sabbath | Steve Thomason
 
Basic Civil Engg Notes_Chapter-6_Environment Pollution & Engineering
Basic Civil Engg Notes_Chapter-6_Environment Pollution & EngineeringBasic Civil Engg Notes_Chapter-6_Environment Pollution & Engineering
Basic Civil Engg Notes_Chapter-6_Environment Pollution & Engineering
 

PCR experiment practice for undergraduate student

  • 1. Class of Modern Life Science Laboratory - May, 2014 - T.A Hong Nhung Nguyen & 서보경 Experiment 10 Polymerase Chain Reaction (PCR)
  • 2. Contents ①Introduction ②Materials and Methods ③Result and Discussion ④Trouble shooting  Purpose of today’s experiment  What is PCR?
  • 3. Purpose of today’s experiment① Introduction www.expeditions.udel.edu Our previous experiments (A) (B) (C) Purpose: Amplify a “DNA fragment of interest” in genomic DNA, total cDNA, plasmid.
  • 4. Dr. Kary Mullis, the inventor of PCR, was awarded the 1993 Nobel Prize in Chemistry. PCR invention and definition① Introduction  PCR is a technique which is used to amplify a specific region of DNA, in order to produce enough DNA to be adequately tested.  A special DNA polymerase (Taq) is used to make many copies of a short DNA fragment (100-10,000 bp) defined by primers.
  • 5. 81,267,844 bp 81,572,676 bp start end ATG10 is located at 5q14.1, size: 304,833 bases Autophagy Related Gene 10 (ATG10) in Chromosome 5 ATG10 …. PCR to amplify a DNA fragment of interest (861 bp) ① Introduction
  • 6. 81,267,844 bp 81,572,676 bp start end ATG10 is located at 5q14.1, size: 304,833 bases ATG10 …. PCR to amplify a DNA fragment of interest (861 bp) Forward and Reverse primers location in genomic DNA
  • 7. for PCR (to amplify a “DNA fragment of interest)Materials and Methods 1. DNA template 2. Primer (10 pmol) 3. Taq DNA Polymerase 4. dNTPs mixture (10 mM) 5. Taq Buffer 10X and 25 mM MgCl2 mixed 6. 5X band doctor (Purchased from Solgent) use only when template DNA is genomic DNA PCR machine 1. DNA (genomic DNA isolated from human or Arabidopsis) Stock concentration: 500 ng/ul 2. cDNA (complementary DNA) synthesize from RNA after Reverse Transcriptase (RT) 3. Plasmid DNA Stock concentration: 50 ug/ul Mixture of Forward and Reverse primer (Listed as detail in your protocol) Stock 5U/ul, speed of synthesize: 1 minute/1 kb
  • 8. Mixture Add DNA template to each sample Experimental design and prepare the mixture PCR machine programming PCR machine Thermocycles
  • 9. Methods Programming Polymerase Chain Reaction Gene Sequence (5’-->3’ direction) Template DNA Tm Expected size(kb) gDNA ATG10-F GAA CAT CCA ATA CTT GGG CAA C MCF-7 gDNA 0.86 ATG10-R AGG GAC ATT TCG TTC ATC CTG 53 53 ? Extension time
  • 10. PCR in test tubes Melting 94 oC Temperature 100 0 50 Time 5’3’ 3’5’
  • 12. PCRMelting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 3’5’ 5’3’ 5’ 5’ Melting 94 oC
  • 13. PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ Heat Heat 5’ 5’ 5’
  • 14. PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’
  • 15. PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’ Heat Heat
  • 16. PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’
  • 17. Fragments of defined length PCR Melting 94 oC Melting 94 oC Annealing Primers 50 oC Extension 72 oC Temperature 100 0 50 Time 30x 3’5’ 5’3’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’ 5’
  • 18.  Why PCR product using cDNA as template sometimes smaller in size? Result PCR using ATG10 F/R specific primer with different templates Where primer should be pick to check mRNA level? 861 bp 207 bp
  • 19. Gene Sequence (5’-->3’ direction) Template DNA Annealing Tm Expected size(kb) gDNA ATG10-F GAA CAT CCA ATA CTT GGG CAA C MCF-7 gDNA 0.86 ATG10-R AGG GAC ATT TCG TTC ATC CTG 53 53 http://genome.ucsc.edu Isoform 1 Isoform 2 Isoform 3 861 bp 207 bp
  • 20. Expected size Common troubles in PCRTroubleshooting Contamination?? Expected size No band?? ??
  • 21. Summary 1. PCR is a technique which is used to amplify a specific region of DNA, in order to produce enough DNA to be adequately tested. 2. PCR is very sensitive 3. PCR need to be well-design and perform in optimal condition Today: Amplify a “DNA fragment of interest” in genomic DNA, total cDNA, plasmid. 861 bp 207 bp