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HUMAN GENOME PROJECT
Presented by,
Rakesh Sharma R
B.Ed .Natural science
Human Genome Project
• Historical context.
• Goals of the HGP.
• Strategy.
• Results.
• Impact on Biomedical domain.
« Finished » sequence
April 1953-April 2003
February 2001
Brief history of HGP
1984 to 1986 – first proposed at US DOE meetings
1988 – endorsed by US National Research Council
(Funded by NIH and US DOE $3 billion set aside)
1990 – Human Genome Project started (NHGRI)
Later – UK, France, Japan, Germany, China
1998. Celera announces a 3-year plan to complete
the project years early
First draft published in Science and Nature in
February, 2001
Finished Human Genome sequence published in
Nature 2003.
Challenges
• Genome Attributes
– Size
– Polymorphism
– Repeats (Smaller repeats are technically difficult to sequence,
some sequences are repeated all over the genome: How can these
be placed?).
• Available Technology
– 600 bp per “read”(Sequencing works by extension from a primer/
gel electrophoresis. Limited by resolution of gel).
– Error (~1 error per 600. Sequencing multiple times decreases
error; same error unlikely in multiple reads. 10x Coverage = error
rate ~1/10,000).
– Relies on cloning (Some regions are difficult to clone
Heterochromatin; some sequences rearrange or are deleted when
cloned)
Goals of HGP
• Create a genetic and physical map of the 24
human chromosomes (22 autosomes, X & Y)
• Identify the entire set of genes & map them all to
their chromosomes
• Determine the nucleotide sequence of the
estimated 3 billion base pairs
• Analyze genetic variation among humans
• Map and sequence the genomes of model
organisms
Model organisms
• Bacteria (E. coli, influenza, several others)
• Yeast (Saccharomyces cerevisiae)
• Plant (Arabidopsis thaliana)
• Roundworm (Caenorhabditis elegans)
• Fruit fly (Drosophila melanogaster)
• Mouse (Mus musculus)
Time-line large scale genomic analysis
Two Competing Strategies for
Human Genome
• (Hierarchical shotgun) [Public human
genome project]
• Whole-genome Shotgun [Celera project]
Sequencing
BAC:
Bacterial Artificial
Chromosome clone
Contig: joined
overlapping collection
of sequences or clones.
Whole-genome shotgun sequencing
Private company Celera used to sequence whole human genome
• Whole genome randomly
sheared three times
– Plasmid library constructed
with ~ 2kb inserts
– Plasmid library with ~10 kb
inserts
– BAC library with ~ 200 kb
inserts
• Computer program assembles
sequences into chromosomes
• No physical map construction
• Only one BAC library
• Reduces problems of repeat
sequences
GenBan
k
DDBJ
EMBL
EMBLEMBL
Entrez
SRS
getentry
NIGNIG
CIB EBI
NCBI
NIHNIH
•Submissions
•Updates •Submissions
•Updates
•Submissions
•Updates
Human genome content
The Human Genome
Total length 3000 Mb
~ 40,000 genes (coding seq)
Gene sequences < 5%
Exons ~ 1.5% (coding)
Introns ~ 3.5% (noncoding)
Intergenic regions (junk) > 95%
Repeats > 50%
Global properties
• Pericentromeric and subtelomeric regions of
chromosomes filled with large recent transposable
elements
• Marked decline in the overall activity of
transposable elements or transposons
• Male mutation rate about twice female
– most mutation occurs in males
• Recombination rates much higher in distal regions
of chromosomes and on shorter chromosome arms
– > one crossover per chromosome arm in each
meiosis
Important features of Human proteome
• 30,000–40,000 protein-coding genes
• Proteome (full set of proteins) more complex than
those of invertebrates.
– pre-existing components arranged into a richer
architectures.
• Hundreds of genes seem to come from horizontal
transfer from bacteria questionable
• Dozens of genes seem to come from transposable
elements.
Noncoding RNA genes
• Transfer RNAs (tRNAs) – adaptors that translate
triplet code of RNA into amino acid sequence of
proteins
• Ribosomal RNAs (rRNAs) – components of
ribosome
• Small nucleolar RNAs (snoRNAs) – RNA
processing and base modification in nucleolus
• Small nuclear RNAs (sncRNAs) - spliceosomes
Human races have similar genes
• Genome sequence centers have sequenced
significant portions of at least three races
• Range of polymorphisms within a race can
be much greater than the range of
differences between any two individuals of
different race
• Very few genes are race specific
• Complexity of proteome increase from
yeast to humans
– More genes
– Shuffling, increase, or decrease of functional
modules
– Alternative RNA splicing – humans exhibit
significantly more
– Chemical modification of proteins is higher in
humans
Yeast
• 70 human genes are known to repair mutations in yeast
•Nearly all we know about cell cycle and cancer comes from
studies of yeast
•Advantages:
•fewer genes (6000)
•few introns
• 31% of yeast genes give same products as human
homologues
Drosophila
• nearly all we know of how mutations affect gene function come
from Drosophila studies
•We share 50% of their genes
•61% of genes mutated in 289 human diseases are found in
fruit flies
•68% of genes associated with cancers are found in fruit flies
•Knockout mutants
•Homeobox genes
C. elegans
• 959 cells in the nervous system
• 131 of those programmed for apoptosis
• apoptosis involved in several human genetic neurological
disorders
•Alzheimers
•Huntingtons
•Parkinsons
Mouse
• known as “mini” humans
•Very similar physiological systems
•Share 90% of their genes
Questions Remain about the
Human Genome
– Difficult to precisely estimate number of genes
at this time
• Small genes are hard to identify
• Some genes are rarely expressed and do not have
normal codon usage patterns – thus hard to detect
Impact of HG on Biomedical
domain
Applications to medicine and
biology
• Disease genes
– human genomic sequence in public databases
allows rapid identification of disease genes in
silico
• Drug targets
– pharmaceutical industry has depended upon a
limited set of drug targets to develop new
therapies
– now can find new target in silico
• Basic biology
– basic physiology, cell biology…
Improve the understanding of disease
etiology and mechanism
Early disease risk assessment
Discover new drug targets
Disease prevention
population or ethnic group variability
The potential benefits of identifying genes/variations
involved in disease
Predisposition
Targeted screening
Prevention
Diagnosis
Therapy
Predictive
medicine
O GOD!
Thank you

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Human genome project

  • 1. HUMAN GENOME PROJECT Presented by, Rakesh Sharma R B.Ed .Natural science
  • 2. Human Genome Project • Historical context. • Goals of the HGP. • Strategy. • Results. • Impact on Biomedical domain.
  • 3. « Finished » sequence April 1953-April 2003 February 2001
  • 4.
  • 5. Brief history of HGP 1984 to 1986 – first proposed at US DOE meetings 1988 – endorsed by US National Research Council (Funded by NIH and US DOE $3 billion set aside) 1990 – Human Genome Project started (NHGRI) Later – UK, France, Japan, Germany, China 1998. Celera announces a 3-year plan to complete the project years early First draft published in Science and Nature in February, 2001 Finished Human Genome sequence published in Nature 2003.
  • 6. Challenges • Genome Attributes – Size – Polymorphism – Repeats (Smaller repeats are technically difficult to sequence, some sequences are repeated all over the genome: How can these be placed?). • Available Technology – 600 bp per “read”(Sequencing works by extension from a primer/ gel electrophoresis. Limited by resolution of gel). – Error (~1 error per 600. Sequencing multiple times decreases error; same error unlikely in multiple reads. 10x Coverage = error rate ~1/10,000). – Relies on cloning (Some regions are difficult to clone Heterochromatin; some sequences rearrange or are deleted when cloned)
  • 7. Goals of HGP • Create a genetic and physical map of the 24 human chromosomes (22 autosomes, X & Y) • Identify the entire set of genes & map them all to their chromosomes • Determine the nucleotide sequence of the estimated 3 billion base pairs • Analyze genetic variation among humans • Map and sequence the genomes of model organisms
  • 8. Model organisms • Bacteria (E. coli, influenza, several others) • Yeast (Saccharomyces cerevisiae) • Plant (Arabidopsis thaliana) • Roundworm (Caenorhabditis elegans) • Fruit fly (Drosophila melanogaster) • Mouse (Mus musculus)
  • 9. Time-line large scale genomic analysis
  • 10. Two Competing Strategies for Human Genome • (Hierarchical shotgun) [Public human genome project] • Whole-genome Shotgun [Celera project]
  • 11. Sequencing BAC: Bacterial Artificial Chromosome clone Contig: joined overlapping collection of sequences or clones.
  • 12. Whole-genome shotgun sequencing Private company Celera used to sequence whole human genome • Whole genome randomly sheared three times – Plasmid library constructed with ~ 2kb inserts – Plasmid library with ~10 kb inserts – BAC library with ~ 200 kb inserts • Computer program assembles sequences into chromosomes • No physical map construction • Only one BAC library • Reduces problems of repeat sequences
  • 14.
  • 15. Human genome content The Human Genome Total length 3000 Mb ~ 40,000 genes (coding seq) Gene sequences < 5% Exons ~ 1.5% (coding) Introns ~ 3.5% (noncoding) Intergenic regions (junk) > 95% Repeats > 50%
  • 16. Global properties • Pericentromeric and subtelomeric regions of chromosomes filled with large recent transposable elements • Marked decline in the overall activity of transposable elements or transposons • Male mutation rate about twice female – most mutation occurs in males • Recombination rates much higher in distal regions of chromosomes and on shorter chromosome arms – > one crossover per chromosome arm in each meiosis
  • 17. Important features of Human proteome • 30,000–40,000 protein-coding genes • Proteome (full set of proteins) more complex than those of invertebrates. – pre-existing components arranged into a richer architectures. • Hundreds of genes seem to come from horizontal transfer from bacteria questionable • Dozens of genes seem to come from transposable elements.
  • 18. Noncoding RNA genes • Transfer RNAs (tRNAs) – adaptors that translate triplet code of RNA into amino acid sequence of proteins • Ribosomal RNAs (rRNAs) – components of ribosome • Small nucleolar RNAs (snoRNAs) – RNA processing and base modification in nucleolus • Small nuclear RNAs (sncRNAs) - spliceosomes
  • 19. Human races have similar genes • Genome sequence centers have sequenced significant portions of at least three races • Range of polymorphisms within a race can be much greater than the range of differences between any two individuals of different race • Very few genes are race specific
  • 20. • Complexity of proteome increase from yeast to humans – More genes – Shuffling, increase, or decrease of functional modules – Alternative RNA splicing – humans exhibit significantly more – Chemical modification of proteins is higher in humans
  • 21. Yeast • 70 human genes are known to repair mutations in yeast •Nearly all we know about cell cycle and cancer comes from studies of yeast •Advantages: •fewer genes (6000) •few introns • 31% of yeast genes give same products as human homologues
  • 22. Drosophila • nearly all we know of how mutations affect gene function come from Drosophila studies •We share 50% of their genes •61% of genes mutated in 289 human diseases are found in fruit flies •68% of genes associated with cancers are found in fruit flies •Knockout mutants •Homeobox genes
  • 23. C. elegans • 959 cells in the nervous system • 131 of those programmed for apoptosis • apoptosis involved in several human genetic neurological disorders •Alzheimers •Huntingtons •Parkinsons
  • 24. Mouse • known as “mini” humans •Very similar physiological systems •Share 90% of their genes
  • 25. Questions Remain about the Human Genome – Difficult to precisely estimate number of genes at this time • Small genes are hard to identify • Some genes are rarely expressed and do not have normal codon usage patterns – thus hard to detect
  • 26. Impact of HG on Biomedical domain
  • 27. Applications to medicine and biology • Disease genes – human genomic sequence in public databases allows rapid identification of disease genes in silico • Drug targets – pharmaceutical industry has depended upon a limited set of drug targets to develop new therapies – now can find new target in silico • Basic biology – basic physiology, cell biology…
  • 28. Improve the understanding of disease etiology and mechanism Early disease risk assessment Discover new drug targets Disease prevention population or ethnic group variability The potential benefits of identifying genes/variations involved in disease Predisposition Targeted screening Prevention Diagnosis Therapy Predictive medicine
  • 30.

Editor's Notes

  1. You all heard the annoncement that the human genome has been sequenced and a first draft was published in February 2001 and a « finished » sequence.
  2. Achievement of this project was compared to the first step of man on the moon
  3. Big deception of the space program, A lot of money to spend some where else, the huge fear from radiation and atomic bomb, main effect cancer, sequence the whole genome, read the book of life.
  4. Before going to the Gene map, genetic maps have been constructed, vectors
  5. Figure 10.13