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Assays to Quantitate Bone Differentiationweek 13

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Transmitted light passed through a solute. Can measure light that has been transmitted or absorbed (by the sample) ... Darker reactions will absorb more light ... – PowerPoint PPT presentation

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Title: Assays to Quantitate Bone Differentiationweek 13


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Assays to Quantitate Bone Differentiationweek 13
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Biojewelry update
  • http//www.biojewelry.co.uk/

4
Spectrophotometry
  • Transmitted light passed through a solute
  • Can measure light that has been transmitted or
    absorbed (by the sample)
  • Darker reactions will absorb more light
  • Ax will be higher
  • A blank is used to eliminate any absorbance
    caused by solvent or buffer
  • Helps determine if there is a contamination or
    cross-reaction in your buffer
  • In our case, PBS used to create lysate

5
Repeat samples
  • Statistically, error is possible
  • Sources of error include
  • Pipetting errors
  • Mixing errors
  • Faults in the plate
  • Plate reader (?)

6
Nomenclature
  • Absorbance is often reported as Al.
  • Transmittance is reported as T
  • Optical Density (OD) is the relationship between
    transmittance and the concentration of the
    colored compound
  • We will only be using Absorbance
  • Compounds created by sample and reagent have
    optimal wavelengths where absorbance occurs.
  • ALP is read at 405nm
  • Calcium is read at 630nm

7
More Nomenclature
  • When you use a well of everything in your sample
    solution MINUS the actual sample this is referred
    to as
  • Blank
  • or Zero
  • or Reference
  • Standards are solutions of known concentration
    used to calibrate the readings

8
ALPalkaline phosphatase
  • p-Nitrophenyl Phosphate is the reagent used to
    indicate concentration of alkaline phosphatase in
    the sample
  • ALP supposed to peak at 2 week and diminish as
    mineral is laid down
  • This assay will determine if this is true or not

9
ALP formula
  • Unit of activity (U/L) -That amount of enzyme
    causing the hydrolysis of one micromole of
    p-nitrophenyl phosphate per minute
  • ALP(U/L) DA/minute X TV X 1000
  • 12.72 X SV
  • TV total volume (0.270ml)
  • 1000 conversion of units from ml to L
  • 12.72 millimolar absorptivity of p-nitrophenol _at_
    405nm _at_ 25oC
  • SV sample volume (variable)
  • Millimolar absorptivity is known so a standard is
    not required
  • PBS sample acts as a zero
  • Not included in calculation

ALP H2O ? Na2HPO4
H
10
Notes for ALP assay
  • This sample is retrieved from entire lysate
  • Note that the sample volumes vary for the
    samples. This changes step 2 on page 110 of the
    manual.
  • This was an adjustment made to keep the readings
    within the parameters of the plate reader.
  • 1 week and undifferentiated 0.01ml
  • 2 week and 3 week 0.005ml

11
Other notes
  • Keep your aliquoted lysates on ice block
  • TA will add RT reagent (p-nitrophenyl phosphate)
  • 1 group/plate
  • Vortex (mixed) lysate sample
  • Timed assay, 0, 2, 4, 6, 8 and 10 minutes
  • Reaction develops over time
  • Also required is Standard Deviation calculation
    for each average
  • Not included in the lab manual at this time
  • X sample absorbance
  • X average absorbance
  • n number of readings

12
Calcium detection
  • Optimal l is 612nm but reading within a range is
    acceptable
  • Requires creation of a linear standard curve
  • Absorptivity of reaction reagent is unknown
  • TA will run standard sample of different
    concentrations for each plate
  • Must run standards each time you run a plate.

13
Calcium assay formula
  • Ca2 of sample (mg/dL)
  • Asample Ablank
  • slope
  • Blank is in well H 1 of each plate
  • There is calcium reagent, but no calcium standard
  • Linear detection range 0.08 mg/dL (0.02mM) to 20
    mg/dL (5mM) calcium in 96-well plate assay.

?
?QuantiChrom Calcium Assay Kit (BioAssay Systems)
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Other notes for Calcium Assay
  • 3 groups/plate since reaction is stable for 60
    minutes
  • Centrifuged supernatant is required sample
  • TA will load standards and all calcium reagent
  • Calcium content should increase over time
    (undifflt1wklt2wklt3wk)

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Cell Migration
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Cell Migration
  • Important in physiological and pathological
    processes
  • Organogenesis and embryonic development
  • Wound healing and angiogenesis
  • Immune system
  • Cancer metastasis
  • Chemotaxis
  • Cell movement in a soluble concentration gradient

17
Tissue Engineering Palsson, Bhatia 2004
These five steps occur after cell is polarized
toward chemoattractant
Thin membrane filaments that are pulled out of
the cell as it moves away are called Retraction
fibers
PtK1 cell
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ECM
  • Cell interactions with ECM exert control over the
    function of the adherent cells
  • Cell spreading, adhesion and migration
  • Surface density of adhesion proteins influences
    the rate of cell migration
  • Too low intracellular contraction forces
    dominate and prevent effective traction against
    the substrate.
  • Too high adhesion strength excessive for cell
    migration, the rear of cell is not released and
    cell speed is reduced

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Tissue Engineering, Minuth, Strehl, Schumacher
2005
Principles of Tissue Engineering, Lanza, Langer,
Vacanti 2000
Tissue Engineering, Minuth, Strehl, Schumacher
2005
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Migrating cell images from 2006
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Measuring cell motility
  • Time lapse microscopy
  • Tracking individuals and populations at fixed
    intervals
  • Specialized migration chambers
  • Before and after measurements by placing cells in
    a starting chamber and counting the cells that
    crawl to another location in a defined period
  • Micropatterning techniques

23
Migration, Boyden Assay
  • Cells above the membrane, chemoattractant is
    below ? concentration gradient
  • Pores 3-8 microns (large enough for the cells to
    squeeze through, small enough so they do not
    fall)
  • Give time to migrate, fix and stain the membrane,
    and count cells at the bottom
  • Disadv cannot trace migration
  • Adv good to view population migration

24
Migration, Zigmond chamber
one well has chemoattractant
cells are under the coverslip, observe them from
the top while migrating
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Migration, Dunn
  • similar to Zigmond in principle, wells are
    concentric as opposed to linear

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Migration, Under agarose
Chemoattractant diffuses through the agarose and
cells migrate out of their well under the agarose
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Cell Migration in Tissue Engineering
  • Polymeric scaffolds created and implanted
  • tissue engineers hope to select certain cell
    types over others
  • Induce enhanced migratory responses of particular
    cell types by
  • Surface chemistry
  • Release of chemoattractants from within the
    implanted material
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