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Identifying cancer selective
            proteins
           Martin McIntosh
    Computational Biology Program
Fred Hutchinson Cancer Research Center
Background
• A variety of alterations in cancer may result in cells encoding proteins or
  polypeptides not observed in normal somatic tissues.

• They may be derived from cancer-related changes in genomes, splicing,
  post-translational modifications, etc.

• These unique disease-related products may be useful for a variety of
  translational goals, including.

    – Therapy: specific targeting of disease tissues.
    – Diagnosis: circulating markers or targets for nanotechnology-based imaging.

• I am going to talk about how we are trying to find these products, and
  implore people (NCI? Others?) to help out.
How we are looking for neoantigen
 candidates: start with RNA-seq.
Central dogma
Central dogma
Central dogma
Central dogma
What do we know about the human
            transcript repertoire
                                                               tissue    normal   cancer
• Un-annotated does not mean it is
  interesting: 15% of splicing events we                       brain     666467   37798
  see in somatic tissues are un-                               testis    165655   1059
  annotated.                                                  placenta   153235     4
                                                                eye      82100      0
                                                               spleen    75504      0
• Annotated!= unimportant: Large bias of                       uterus    70546    35040
  cancer tissues populate the EST                              blood     69245    24036
                                           normal
  databases.             cancer
                                                               kidney    63980    30706
                                                                lung     63495    32601
               Few Samples:                                   thymus     62142      0
                                                              pancreas   59037    25447
                                                               muscle    55891    9730
                                                               heart     53531      0
                                                                liver    52532    36124
                                                              prostate   43049    11959
               More Samples:
                                                               ovary      8413    26755


                                                    UCSC EST Libraries (those that
                                                    map to human tissues): Characterized
                                                    by organ/tissue and development stage.
Example of putative “Novel” protein




Left: A four nucleotide extension and alternate exon for SF1 which together cause
frame shift that maintains the stop codon in the terminal exon. Right: Confirmation
of spectra by comparing tumor (red) to synthetic spectra (blue). Confirmed by
sequencing.
Why not use MS proteomics?

              MS/MS=Matching technology

              Low sensitivity compared to RNAseq.

              Low coverage per protein identified.




                   Biology gets in the way.

                   Exon-exon boundaries frequently
                   cut by trypsin.
Cancer selective splicing events across
            disease sites
Figure 2: (Left): Clustering of prevalent and abundant cancer selective transcripts to known CT
antigens observed in ovarian cancer tissues, a subset of 112 known tumor selective transcripts
identified. (Right): A tandem 3’ splice site, with a NAGNAG motif, in BRCA1, is observed in ovarian
(top) and prostate (bottom) cancer, in normal testis, but no other normal or control RNA-Seq data or
normal ESTs. Figure shows splice viewer our group developed.

  Right panel shows splicing viewer developed into IGV (broad) by my group (Damon May).
Lots of changes do not result in code
How we are trying to improve the
           pipeline.
                Specificity to tumor cells:
                • Many putative coding
                  sequences may be un-
                  annotated species
                  belonging to infiltrating
                  cells.
                • We are creating single-cell
                  suspensions and separating
                  tumor cells from other cells,
                  and sequencing each
                  component.
How we are trying to improve pipeline

                                                                                        Specificity for coding sequences
• Separa on following sucrose ultracentrifuge.                                          • Enrich for mRNA’s
                                                                                          undergoing active
                               Derived from Ovcar 3 Cell Line
                      A
                          ?"
                                             B                       C
                                                                                          translation.
      Ribosomes+
      Transcript/ribosome

                            M$
                                                                                        • Capture polysome-bound
                                      2$         3$   4$   5$   6$       7$   8$   9$
                                                                                          transcripts.
                   40S$ 60S$ 80S$
                                     120S$



            Number of ribosome's bound: as measured by op cal readout.
What exactly do we mean by a protein coding gene?



           A



           B



           C




     Result from one mouse pool (mouse heart). Actin beta, including
     annotated exon known to be selected for NSMD.

     Brings up an epistemological issue for proteomics people
Is it really sufficient that we see ribosomes?




       Non-coding RNA (Malat1) found in mouse heart.
       Pronounced with 2 or 3 ribosomes .

       Interested in looking at ribosome foot printing
Summary
• Who cares about a millions of genomes.
• Genomes looks to me like an engineering
  problem and not really a research problem.
• Relying on changes in proteins derived solely
  from changes in cancer genomes (e.g.,
  mutations) may not provide a large number of
  putative candidates.
• MS proteomics does not work well enough, RNA-
  seq works too well.
• We need someone to begin to better characterize
  the nucleotides contained in somatic tissues.
Credit
•   People who did the work:
     – Matt Fitzgibbon (Computational lead).
     – Nigel Clegg (visual curation and EST database).
     – Damon May (IGV Visual curation).
     – Lindsay Bergen (all Laboratory work).

•   Funding:
     – No. HHSN261200800001E: NCI in-Silico Center of Excellence
     – Canary Foundation.
     – Illumina
•   Thanks:
     – Vivian MacKay (UW Biochem), polysome fractionation.
     – Nicole Urban, Chuck Drescher, FHCRC Ovarian SPORE.

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Dr. Martin McIntosh: Identifying Cancer Selective Proteins Using RNA-Sequencing and Bioinformatics Strategies

  • 1. Identifying cancer selective proteins Martin McIntosh Computational Biology Program Fred Hutchinson Cancer Research Center
  • 2. Background • A variety of alterations in cancer may result in cells encoding proteins or polypeptides not observed in normal somatic tissues. • They may be derived from cancer-related changes in genomes, splicing, post-translational modifications, etc. • These unique disease-related products may be useful for a variety of translational goals, including. – Therapy: specific targeting of disease tissues. – Diagnosis: circulating markers or targets for nanotechnology-based imaging. • I am going to talk about how we are trying to find these products, and implore people (NCI? Others?) to help out.
  • 3. How we are looking for neoantigen candidates: start with RNA-seq.
  • 8. What do we know about the human transcript repertoire tissue normal cancer • Un-annotated does not mean it is interesting: 15% of splicing events we brain 666467 37798 see in somatic tissues are un- testis 165655 1059 annotated. placenta 153235 4 eye 82100 0 spleen 75504 0 • Annotated!= unimportant: Large bias of uterus 70546 35040 cancer tissues populate the EST blood 69245 24036 normal databases. cancer kidney 63980 30706 lung 63495 32601 Few Samples: thymus 62142 0 pancreas 59037 25447 muscle 55891 9730 heart 53531 0 liver 52532 36124 prostate 43049 11959 More Samples: ovary 8413 26755 UCSC EST Libraries (those that map to human tissues): Characterized by organ/tissue and development stage.
  • 9. Example of putative “Novel” protein Left: A four nucleotide extension and alternate exon for SF1 which together cause frame shift that maintains the stop codon in the terminal exon. Right: Confirmation of spectra by comparing tumor (red) to synthetic spectra (blue). Confirmed by sequencing.
  • 10. Why not use MS proteomics? MS/MS=Matching technology Low sensitivity compared to RNAseq. Low coverage per protein identified. Biology gets in the way. Exon-exon boundaries frequently cut by trypsin.
  • 11. Cancer selective splicing events across disease sites
  • 12. Figure 2: (Left): Clustering of prevalent and abundant cancer selective transcripts to known CT antigens observed in ovarian cancer tissues, a subset of 112 known tumor selective transcripts identified. (Right): A tandem 3’ splice site, with a NAGNAG motif, in BRCA1, is observed in ovarian (top) and prostate (bottom) cancer, in normal testis, but no other normal or control RNA-Seq data or normal ESTs. Figure shows splice viewer our group developed. Right panel shows splicing viewer developed into IGV (broad) by my group (Damon May).
  • 13. Lots of changes do not result in code
  • 14. How we are trying to improve the pipeline. Specificity to tumor cells: • Many putative coding sequences may be un- annotated species belonging to infiltrating cells. • We are creating single-cell suspensions and separating tumor cells from other cells, and sequencing each component.
  • 15. How we are trying to improve pipeline Specificity for coding sequences • Separa on following sucrose ultracentrifuge. • Enrich for mRNA’s undergoing active Derived from Ovcar 3 Cell Line A ?" B C translation. Ribosomes+ Transcript/ribosome M$ • Capture polysome-bound 2$ 3$ 4$ 5$ 6$ 7$ 8$ 9$ transcripts. 40S$ 60S$ 80S$ 120S$ Number of ribosome's bound: as measured by op cal readout.
  • 16. What exactly do we mean by a protein coding gene? A B C Result from one mouse pool (mouse heart). Actin beta, including annotated exon known to be selected for NSMD. Brings up an epistemological issue for proteomics people
  • 17. Is it really sufficient that we see ribosomes? Non-coding RNA (Malat1) found in mouse heart. Pronounced with 2 or 3 ribosomes . Interested in looking at ribosome foot printing
  • 18. Summary • Who cares about a millions of genomes. • Genomes looks to me like an engineering problem and not really a research problem. • Relying on changes in proteins derived solely from changes in cancer genomes (e.g., mutations) may not provide a large number of putative candidates. • MS proteomics does not work well enough, RNA- seq works too well. • We need someone to begin to better characterize the nucleotides contained in somatic tissues.
  • 19. Credit • People who did the work: – Matt Fitzgibbon (Computational lead). – Nigel Clegg (visual curation and EST database). – Damon May (IGV Visual curation). – Lindsay Bergen (all Laboratory work). • Funding: – No. HHSN261200800001E: NCI in-Silico Center of Excellence – Canary Foundation. – Illumina • Thanks: – Vivian MacKay (UW Biochem), polysome fractionation. – Nicole Urban, Chuck Drescher, FHCRC Ovarian SPORE.