Presentation is loading. Please wait.

Presentation is loading. Please wait.

The 454 and Ion PGM at the Genomics Core Facility Dr. Deborah Grove, Director for Genetic Analysis Genomics Core Facility Huck Institutes of the Life Sciences.

Published byHeather Ross Modified over 9 years ago

Similar presentations

Presentation on theme: "The 454 and Ion PGM at the Genomics Core Facility Dr. Deborah Grove, Director for Genetic Analysis Genomics Core Facility Huck Institutes of the Life Sciences."— Presentation transcript:

1 The 454 and Ion PGM at the Genomics Core Facility Dr. Deborah Grove, Director for Genetic Analysis Genomics Core Facility Huck Institutes of the Life Sciences Penn State University

2 Services DNA Sequencing Illumina, 454 and Ion PGM Next Gen Sequencing Microarray Genotyping – VNTRs, SNPs, Open Array qPCR by Real-Time DNA Synthesis DNA Extraction and Storage of DNA from Buccal Swabs

3 Sequencing at PSU Over the Years MethodManual Gel Bases per Day 1200

4 Cycle Sequencing Reaction

5 Sequencing at PSU Over the Years MethodManual Gel 377 Gel Bases per Day 120020,000

6 Sequencing at PSU Over the Years MethodManual Gel 377 Gel3100 –16 Capillary Bases per Day 1200?20,000100,000

7 Sequencing at PSU Over the Years MethodManual Gel 377 Gel3100 –16 Capillary 3730--96 Capillary Bases per Day 1200?20,000100,0000.5 to 1 million

8 Sequencing at PSU Over the Years MethodManual Gel 377 Gel3100 –16 Capillary 3730--96 Capillary SOLiD Next-Gen Bases per Day 1200?20,000100,0000.5 to 1 million 1 to 2 Billion

9 Next-Generation Sequencers: Massively Parallel Platforms Roche 454FLX+ v2.8 – 500 million bases per run, 800 to 1000 bases Ion PGM 318 chip – 2 to 4 billion bases per run, 400 base length (Ion Proton)

10 Roche 454 – Next Generation Sequencer Pyrosequencing FLX+ v2.8 has 800 to 1000 bp read 160 million bases per full slide 454 FLX +

11 454 Titanium Sequencing Applications Transcriptome RNA Whole Genome -- Paired-End (3kb, 8kb, 20kb) 15 to 30 ugs dsDNA Whole Genome – Shotgun 500 ngs dsDNA Amplicon/Metagenomics 5 ngs

12 DNA Fragmentation by nebulization Fragment End Repair AMPure Bead Clean up Adaptor-Ligation Small Fragment Removal Library Quality Assessment and Quantification

13

14

15 Primer Sets for Metagenomics 16s Bacteria ITS for Fungus 18s set for Fungus and other Eukaryotes, targeting Protists Archaea targeting both Crenarchaeota and Euryarchaeota

16 Amplicon Preparation 27F_M6CGTATCGCCTCCCTCGCGCCATCAGATATCGCGAGAGAGTTTGATCMTGGCTCAG 907R_M6TATGCGCCTTGCCAGCCCGCTCAGCCCCGTCAATTCMTTTGAGTTT

17 16S Variable Regions 27F_M6CGTATCGCCTCCCTCGCGCCATCAGATATCGCGAGAGAGTTTGATCMTGGCTCAG 907R_M6TATGCGCCTTGCCAGCCCGCTCAGCCCCGTCAATTCMTTTGAGTTT

18 Amplicons 27F 518R 907R

19

20 One Bead One DNA library NTPs, Taq etc.

21

22

23

24

25

26

27

28

29 Ion PGM aka Ion Torrent

30 314 CHIP316 CHIP

31 Approximate Cost from Genome Library thru Sequencing 314 Chip160 million bases, 400,000 reads 318 Chip3 billion bases, 6 to 8 million reads $1500 to $2000

32 Coverage Full Plate = 1 million reads, 300 million bases ½ plate = 500,000 reads, 150 million bases 1 Quad = 200,000 reads, 60 million bases

33 Coverage

34 Full Plate = 1 million reads, 300 million bases ½ plate = 500,000 reads, 150 million bases 1 Quad = 200,000 reads, 60 million bases http://www.youtube.com/embed/yVf2295JqUg

35 Coverage Full Plate = 1 million reads, 300 million bases ½ plate = 500,000 reads, 150 million bases 1 Quad = 200,000 reads, 60 million bases

36 Full Plate = 1 million reads, 300 million bases ½ plate = 500,000 reads, 150 million bases 1 Quad = 200,000 reads, 60 million bases

37 Full Plate = 1 million reads, 300 million bases ½ plate = 500,000 reads, 150 million bases 1 Quad = 200,000 reads, 60 million bases

38 Applications Bacterial and Viral Genomes Amplicons Ampliseq Panels for SNP variants

39 Ampliseq Cancer Panel Only 10 ngs or less FFPE tissues Single Cells Libraries take 3.5 hours 2800 hot spots

40 Ampliseq Custom Panels Use Ion AmpliSeq Designer

41

42 P1 Chip 80 million reads, 10 to 15 billion bp PII Chip 300 million reads, 500 to 800 billion bp 314 Chip 160 million bases, 400,000 reads 318 Chip 3 billion bases, 6 to 8 million reads

43 Pac Bio No amplification required Single molecule Several thousand base reads (4 to 20 kb) Least GC-biased sequencing Run time 30 minutes

44 Genomes: Finish Genomes and improve assembly with extra long reads (4000bp average and up to 20,000) Genomic Complexity: Allow haplotype expansion, full length transcripts and splice variants, repeat expansions, minor variants Epigenome: Detects base modifications using kinetics Applications

45 Thanks to: The Huck Institutes of the Life Sciences Lloyd and Dorothy Huck And the others in the lab…

Download ppt "The 454 and Ion PGM at the Genomics Core Facility Dr. Deborah Grove, Director for Genetic Analysis Genomics Core Facility Huck Institutes of the Life Sciences."

Similar presentations

Next-Generation Sequencing: Methodology and Application

Next-Generation Sequencing: Methodology and Application
High throughput sequencing Barbera van Schaik

High throughput sequencing Barbera van Schaik
Schulich School of Medicine & Dentistry The University of Western Ontario London Regional Genomics Centre Next Generation Sequencing Meeting April 1, 2010.

Schulich School of Medicine & Dentistry The University of Western Ontario London Regional Genomics Centre Next Generation Sequencing Meeting April 1, 2010.
The Past, Present, and Future of DNA Sequencing

The Past, Present, and Future of DNA Sequencing
The Good, Bad, and Ugly of Next-Gen Sequencing

The Good, Bad, and Ugly of Next-Gen Sequencing
 Sequencing technology › Roche/454 GS-FLX (‘454’) › Illumina  Prokaryotic profiling › De novo genome sequencing › Metagenomics › SNP profiling › Species.

 Sequencing technology › Roche/454 GS-FLX (‘454’) › Illumina  Prokaryotic profiling › De novo genome sequencing › Metagenomics › SNP profiling › Species.
Next–generation DNA sequencing technologies – theory & practice

Next–generation DNA sequencing technologies – theory & practice
Next-generation sequencing

Next-generation sequencing
The past, present, and future of DNA sequencing Dan Russell.

The past, present, and future of DNA sequencing Dan Russell.
What Is Genomics? Genomics is the study of how the entire genome of a species functions as a unit and evolves over time. It is the study of life’s blueprint,

What Is Genomics? Genomics is the study of how the entire genome of a species functions as a unit and evolves over time. It is the study of life’s blueprint,
Next-generation sequencing and PBRC. Next Generation Sequencer Applications DeNovo Sequencing Resequencing, Comparative Genomics Global SNP Analysis Gene.

Next-generation sequencing and PBRC. Next Generation Sequencer Applications DeNovo Sequencing Resequencing, Comparative Genomics Global SNP Analysis Gene.
Greg Phillips Veterinary Microbiology gregory@iastate.edu.

Greg Phillips Veterinary Microbiology
The SOLiD System: Next-Generation Sequencing Overview of the SOLiD System –  Scalable  Accurate Ultra High Throughput  Flexible  Mate Pairs.

The SOLiD System: Next-Generation Sequencing Overview of the SOLiD System –  Scalable  Accurate Ultra High Throughput  Flexible  Mate Pairs.
High Throughput Sequencing

High Throughput Sequencing
CS 6293 Advanced Topics: Current Bioinformatics

CS 6293 Advanced Topics: Current Bioinformatics
Genome Sequencing and Assembly High throughput Sequencing Xiaole Shirley Liu STAT115, STAT215, BIO298, BIST520.

Genome Sequencing and Assembly High throughput Sequencing Xiaole Shirley Liu STAT115, STAT215, BIO298, BIST520.
1 100 120 University of Oklahoma Genome Center4/14/12.

University of Oklahoma Genome Center4/14/12.
Cancer Genomics Lecture Outline

Cancer Genomics Lecture Outline
Diabetes and Endocrinology Research Center The BCM Microarray Core Facility: Closing the Next Generation Gap Alina Raza 1, Mylinh Hoang 1, Gayan De Silva.

Diabetes and Endocrinology Research Center The BCM Microarray Core Facility: Closing the Next Generation Gap Alina Raza 1, Mylinh Hoang 1, Gayan De Silva.
Zachary Bendiks. Jonathan Eisen  UC Davis Genome Center  Lab focus: “Our work focuses on genomic basis for the origin of novelty in microorganisms (how.

Zachary Bendiks. Jonathan Eisen  UC Davis Genome Center  Lab focus: “Our work focuses on genomic basis for the origin of novelty in microorganisms (how.

Similar presentations

Ads by Google