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Test system for systems biology

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Test system for systems biology Four distinct types of global datasets were generated and analyzed Proteome analysis quantitative proteomics (ICAT technology) to ... – PowerPoint PPT presentation

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Title: Test system for systems biology


1
Test system for systems biology
  • Four distinct types of global datasets were
    generated and analyzed
  • Proteome analysis quantitative proteomics (ICAT
    technology) to analyze 300 proteins in wild-type
    yeast with the system turned on and off
  • Thirty of these proteins changed in the
    transition between these two biological states
  • the mRNA and protein changes went in different
    directions for 15 of these examples
  • post-transcription control mechanisms must
    regulate protein synthesis in half of the examples

2
Test system for systems biology
  • Four distinct types of global datasets were
    generated and analyzed
  • Kinetic analysis of global mRNA concentrations
    change across the physiological time span of
    activation of the galactose biomodule
  • Kinetic data provide powerful new approaches to
    understanding the temporal operation of the
    galactose biomodule and its temporal connections
    to other biomodules in the yeast cell

3
Test system for systems biology
  • Endomesodermal development in sea urchin
  • The architecture of a gene regulatory network is
    specified by the DNA binding sites, for these
    establish the linkages of the transcription
    factors that coordinate the behaviors of genes
    throughout the gene regulatory networks.
  • The gene regulatory networks contribute to
    determine the behavior of the peripheral
    (structural) genes in the network.
  • The peripheral genes ultimately execute the
    specific development functions that underlie
    particular aspects of development.

4
  • The green panel depicts primarily transcription
    factors and their interactions with the control
    regions of other transcription factors.
  • Genes are indicated by horizontal lines.
  • Arrowheads indicate activation.
  • I indicate repression
  • The yellow (lower) panel indicates peripheral
    genes that carry out the functions of endodermal
    development.

5
  • The 2.1-kb promoter region of the endo16 gene is
    enlarged here and depicts 34 DNA binding sites
    (rectangles) and 13 different transcription
    factors and cofactors (rectangles or lollipops
    connected by lines to the DNA binding sites).
  • Experiments indicate that there are six modules
    (AG) that carry out discrete functions for the
    developmental regulation of endo 16.
  • The ultimate objective is to convert this logic
    diagram into a mathematical formulation that
    accurately represents the subtle complexities of
    this developmental circuit.

6
  • A logical diagram depicting the functions of the
    A and B modules throughout endomesodermal
    development.
  • This logic then embodies a mathematical
    relationship between the control segments.

7
Hostpathogen systems biology
  • For tryptophan biosynthesis C. psittaci obtains
    an alternative source of anthranilate by
    hijacking the hosts tryptophan depletion pathway
    by intercepting the byproduct kynurenine.
  • the tryptophan depletion pathway of the host is
    activated by inducing indoleamine-2,3-dioxygenase
    using IFN-?
  • C. psittaci uses host kynurenine through kynU to
    produce its own tryptophan, enabling
    intracellular growth and causing chronic
    infections.

8
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9
Hostpathogen systems biology
  • Group A Streptococcus, the causative agent of
    mild infections and life-threatening invasive
    diseases, produces many virulence factors that
    promote survival in humans.
  • A two component regulatory system, designated
    covRS (cov, control of virulence csrRS),
    negatively controls expression of five proven or
    putative virulence factors (capsule, cysteine
    protease, streptokinase, streptolysin S, and
    streptodornase)
  • Inactivation of covRS results in enhanced
    virulence in mouse models of invasive disease

10
  • GAS CovR gene regulation network delineated by
    microarray expression analysis. CovRS respond to
    unknown environmental signals and modulate
    expression of several broad categories of GAS
    genes involved in growth and adaptation by a
    phosphorelay mechanism. CovR-regulated gene
    products influence hostpathogen interactions,
    including capsular polysaccharide (capsule), cell
    proteins anchored via LPXTG motifs (surface
    proteins), cytosolic and membrane proteins
    involved in environmental adaptation (adaptation
    response), and extracellular proteins containing
    secretion signals (secreted proteins).
  • Several two-component systems (ovals) and other
    transcriptional regulators (squares) are also
    CovR-regulated, but their downstream regulatory
    consequences are unknown. Red lines,
    down-regulation green lines, up-regulation. PG,
    peptidoglycan, secreted proteins surface solid
    rectangles, secreted proteins with LPXTG motifs.
    Numbers denote SPy numbers assigned for serotype
    M1 GAS strain SF370 ORFs.

11
Hostpathogen systems biology
  • Systems biology in malaria research integrating
    genomics, transcriptomics and proteomics, we can
  • classify and annotate genes by their expression
    profiles
  • detect evidence of posttranscriptional gene
    silencing in the murine malaria species.
  • Metabolic pathway reconstruction by expression
    analysis

12
  • Metabolic pathway reconstruction by expression
    analysis.
  • (a) Table showing representation of protein
    expression from the glycolytic and TCA pathways,
    color coded by protein sequence coverage
    identified through proteomics experiments (see
    key). The sequence coverage values in the table
    serve as a crude measurement of protein
    abundance. Values are from Ref. 1. During
    asexual blood stages, the glycolytic pathway is
    active, resulting in the production of lactate,
    whereas there is no evidence of a complete TCA
    cycle during these stages.
  • (b) Pathway glyph representation of the activity
    of metabolic pathways, as determined by their
    proteomics expression profiles.Red indicates
    active pathways and gray indicates inactive
    pathways.

13
Hostpathogen systems biology
  • Systems biology in Schistosoma research
    integrating genomics, transcriptomics and
    proteomics
  • Reconstruction and in silico analysis of the MAPK
    and WNT signaling pathways in Schistosoma
    japonicum
  • MAPK signaling pathways regulating
    proliferation and differentiation processes in
    Schistosoma

14
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15
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16
Hostpathogen systems biology
  • The global molecular interaction architecture of
    the immune system
  • molecular interactions of the immune system
    actually consist of a nested tandem bow-tie
    architecture
  • This architecture can be recognized both in
    intracellular signal transduction pathways and in
    intercellular signaling processes

17
  • Nested bow-tie architecture in immune system.
    Salient features of the immune system network are
    nested bow-tie structures and extensive feedback
    loops. The bow-tie structure of intercellular
    interactions

18
  • The bow-tie architecture also exists at the
    signal transduction level

19
Future directions or open issues in systems
biology
  • Nanotechnology
  • integration across disciplines
  • Modeling

20
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