PROLIFERATIVE VITREORETINOPATHY: ARRAY OR DISARRAY - PowerPoint PPT Presentation

1 / 47

About This Presentation

Title:

PROLIFERATIVE VITREORETINOPATHY: ARRAY OR DISARRAY

Description:

PROLIFERATIVE VITREORETINOPATHY: ARRAY OR DISARRAY – PowerPoint PPT presentation

Number of Views:1079

Avg rating:3.0/5.0

Slides: 48

Provided by: Asatisfied321

Category:

more less

Transcript and Presenter's Notes

Title: PROLIFERATIVE VITREORETINOPATHY: ARRAY OR DISARRAY

1
PROLIFERATIVE VITREORETINOPATHY ARRAY OR DISARRAY
2
OUTLINE

Introduction
Structure of Retina
Proliferative Vitreoretinopathy
cDNA macroarrays
Real time PCR
cDNA microarrays
Future Work

3
ANATOMY OF THE EYE
http//webvision.med.utah.edu/sretina.html
4
CROSS-SECTION OF RETINA
CHOROID
http//webvision.med.utah.edu/sretina.html
VITREOUS
5
FUNCTIONS OF RPE
choroid

Barrier epithelium
Reduce light scattering
Visual cycle
Phagocytosis
Keeps the retina attached

vitreous
6
CHARACTERISTICS OF RPE

Normally non-dividing
But can divide
tissue culture
pathological conditions

7
PROLIFERATIVE VITREORETINOPATHY (PVR)

Tear/damage in retina
RPE cells lose contact inhibition
Cells gain access to vitreous
Proliferate
Make extracellular matrix (ECM)

8
PVR (CONTD.)

RPE cells attach to collagen fibers and other
components of the ECM
Epiretinal membranes formed
Migration/attachment - tangential force on the
retina
Anterior and posterior vitreous cortex contracts
Retinal detachment

9
RISK FACTORS FOR PVR

Retinal holes, retinal breaks or retinal tears
(eye trauma )
RPE cells in vitreous
Breakdown of blood-retinal barrier and/or
inflammation
Mechanical forces on retina - traction
Hereditary abnormalities of peripheral retina
-myopia

10
FORMATION OF EPIRETINAL MEMBRANES
Liou G, unpublished results
11
CLINICAL IMPORTANCE

In the US and Worldwide 5-10 of retinal
detachment is due to PVR
Surgical treatment not very effective
Past approach in the treatment of PVR has been
disappointing
Need to develop new therapeutic agents

12
EPITHELIAL-MESENCHYMAL TRANSFORMATION (EMT)

Transformation occurs in development and disease
Epithelial cells undergoing EMT
lose cell-cell and cell-basement membrane
interactions
fibroblast-like morphology
become mobile
proliferative and invasive
Very similar to changes that occur during
tumor formation

13
VITREOUS HUMOR AND PVR

Vitreous shown to contribute to EMT in cultured
RPE
RPE cells with fibroblast morphology cause
contraction of the collagen gel in a model system.

14
Effect of Vitreous on the Morphology of RPE Cells
B
A
CONTROL
25 VITREOUS
15
VITREOUS

Gel
Collagen fibers in hyaluronic acid matrix
Collagen II
some collagen V/XI, VI, IX
Also contains variety of other components
transferrin, albumin
chemotactic factors, growth factors and
morphogenic factors, matrix metalloproteinases
etc

16
WHAT DO WE KNOW ABOUT PVR-MOLECULAR LEVEL?

HOW SHOULD WE APPROACH THIS PROBLEM?
Detachment
Motility
Invasiveness
ECM formation
Contraction

17
APPROACHES TO IDENTIFICATION OF MOLECULAR LESIONS

Individual gene approach
RT-PCR
Northern blots
Western blots
Global approach
cDNA macroarrays
cDNA microarrays

18
MACROARRAYS

Clontech
Postively charged nylon membrane (588 double
spots)
Isotope (p-32)
Expose to film and develop (1-10 days)

19
cDNA MACROARRAY (10 day exposure)
20
Change in mPGES and MMP-14 RNA Expression after
Incubation of RPE cells with Vitreous
PGES
PGES
MMP-14
MMP-14
21
QUICK CHECK FOR DNA CONTAMINATION
22
REAL TIME PCR VALIDATION
Real-time PCR analyses RPLPO and PGES
Control cells
Vitreous-treated cells
23
OTHER GENES VALIDATED

Alpha-5 integrin
MMP-14
COX-2

24
LIMITATIONS

Why switch from membranes to glass slides?
Some limitations of membrane arrays
Expensive
Fewer genes represented
Control and experimental samples on different
membranes
Bleeding from adjacent spots very common problem
High background

25
GLASS SLIDE ARRAYS or MICROARRAYS

Probe is tethered to an immobile surface, such as
glass
Glass durable, non-porous, allows covalent
attachment of probe
Probe spotted by pins or capillary tubes
Low background fluorescence

26
GLASS SLIDE ARRAYS or MICROARRAYS (CONTD.)

Sample hybridized to array
Detected by fluorescence
At least two fluorochromes used, cy3 and cy5 i.e,
simultaneous hybridization
Massive amounts of data generated (data mining)

27
DISADVANTAGES

Limitations of microarrays
Large amounts of starting RNA required
Stability problems with light exposure
Need laser scanner
Current location of scanner

28
PREPARATION OF TARGET PROBE
DIRECT and INDIRECT LABELING
Direct incorporation of cy3/cy5 labeled dCTP
during RT, i.e enzymatic incorporation
RT using aminoallyl dUTP (amine modified analog
of dUTP) Post labeling with cy3/cy5 coupled to
NHS ester
29
cDNA AMPLIFICATION

At least 100ug of total RNA needed
Amplification necessary
Eberwine method using the T7 system

30
DISADVANTAGES OF PCR LABELING OVER T7

Skewing of population is more because it is
logarithmic over linear skewing using T7
As a result of logarithmic skewing some RNAs
might never be represented in the PCR system

31
AMBION T7 AMPLIFICATION
RT
RT
First strand cDNA synthesis
pol
X?X?X?
Rnase H digestion products - primer
Double strand cDNA
pol
pol
pol
pol
Copied strands are anti-sense to original mRNA
aRNA
32
CYSCRIBE DIRECT LABELING PROTOCOL

Take 1ug aRNA from T7 amplification
RT using cy3/cy5 labeled dCTP
Purify and concentrate
Hybridize 14-16hrs in 37C incubator
Wash 3 times with high and low salt
Scan using Packard Scanner at RMH

INCORPORATION OF DYES DURING RT
33
POINTS TO REMEMBER

Control and experimental sample
Labeled with two fluors
Hybridized to same microarray
False color palette
Red-cy3, green cy-5
Yellow-equal representation of cDNA in both
samples

34
CYSCRIBE DIRECT LABELING
1.7k gene array
35
CYSCRIBE DIRECT LABELING
36
AMBION POST LABELING PROTOCOL

Take 1ug aRNA from T7 amplification
RT using Ambion amino allyl kit (aadUTP)
Couple with NHS form of cy3/cy5
Purify and concentrate
Hybridize 14-16hrs in 37C incubator
Wash 3 times with high and low salt
Scan using Packard Scanner at RMH

INCORPORATION OF DYES AFTER RT
37
AMBION POST LABELING
38
AMBION POST LABELING
39
COMPARISON OF DIRECT AND POST LABELING

Very similar over all results

40
UPSCALING TO 20K GENE ARRAYS

University of Toronto (OCI)
20000 genes double spotted on two slides

Control epithelial cells Experimental
mesenchymal cells ( vitreous) Time course 0-48
hours Labeling method direct
41
20K GENE ARRAY
20K GENE ARRAY SLIDE A
20K GENE ARRAY SLIDE B
42
Vitreous
6hr
12hr
24hr
48hr
Epithelial Cuboidal Polarized Adherent Non-motile
Fibroblastic Elongated Non-polarized Separated Mot
ile
Loss of shape
Overgrowth
Signals Receptors Transcription factors
Cytoskeletal Changes Actin - keratin
Intercellular Adherent Protein changes ECM-integri
n changes Motility proteins
Possible Changes
43
ADHESION/SKELETAL PROTEINS IN FIRST 20K GENE ARRAY
Vitreous
6hr
12hr
24hr
48hr
Epithelial Cuboidal Polarized Adherent Non-motile
Fibroblastic Elongated Non-polarized Separated Mot
ile
Loss of shape
Overgrowth
Signals Receptors Transcription factors
Cytoskeletal Changes Actin - keratin
Intercellular Adherent Protein changes ECM-integri
n changes Motility proteins

NR CAM
Alpha 3 integrin (proteome)
Zyxin (adherens junction of RPE)
Contactin
Cadherin 8
Proteoglycan-2
Myosin SMA
Alpha 2 actin
Gamma 2 actin

Alpha 5 integrin (proteome)
Restin (int filament)
Lamin B receptor
Transmembrane protease ser-4 (in tumor
progression)

Adhesion proteins UP at 24 hours
Adhesion proteins DOWN at 24 hours
44
SIGNALING PROTEINS
Vitreous
6hr
12hr
24hr
48hr
Epithelial Cuboidal Polarized Adherent Non-motile
Fibroblastic Elongated Non-polarized Separated Mot
ile
Loss of shape
Overgrowth
Signals Receptors Transcription factors
Cytoskeletal Changes Actin - keratin
Intercellular Adherent Protein changes ECM-integri
n changes Motility proteins