How to visualize genes
and their products
Kamil Růžička
FGP CEITEC MU
Genomics Lectures Series
Outline
• reporter genes
• promoter fusions
• visualizing proteins
• visualizing RNA
• dynamics of protein imaging: FRAP,
photoactivable proteins, FLIM, FCS
Promoter activity monitoring
promoter here can be reporter terminator
1-10 kb prior to ATG
LacZ, GUS
Luciferase
GFP
Reporter genes
• LacZ, GUS
• Luciferase
• GFP
some need external substrate, some not
LacZ, GUS – rhapsody in blue
(in case of GUS – X-Gluc)
promoter LacZ terminator
soluble
insoluble
LacZ, GUS
LacZ/ GUS:
worm, mouse – LacZ, plants - GUS
Luciferase
(used principle of chemiluminiscence)
promoter luciferase terminator
What’s difference between flurescence and luminiscence?
Luciferase
How does fluorescence work?
energy
How does a fluorescence
microscope work?
Stokes shift
George G. Stokes
How does a confocal
microscope work?
What are advantages of confocal microscopy?
Live imaging
Martin Chalfie
GFP discovery - Nobel Prize 2008
Roger TsienOsamu Shimomura
Many fluorescent proteins on
the market (Tsien’s fruits)
Excitation and emission
Multicolored fluorescent protein
image (neurones)
Promoter-GFP
promoter GFP terminator
Promoter activity monitoring
choice of suitable reporter
• LacZ, GUS
• Luciferase
• GFP
accessibility, sensitivity, accuracy…
Promoter activity monitoring
• LacZ, GUS
– easy assay, also on sections, easy imaging
– substrate must diffuse, kills the organism
• luciferase
– good quantification, very sensitive, no
autophluorescence
– substrate must diffuse, special machine, dark
• GFP
– good sensitivity, colocalization with other
dyes/promoters possible, no substrate needed
– only in vivo, autophluorescence, thin transparent
sample; it should be ER localized in plants
Luminiscent mouse better
than phluorescent mouse
Promoter activity monitoring
Pros:
•
Cons:
•
Promoter activity monitoring
Pros:
• easy to clone, easy to visualize
• usually some signal seen – cheers you up!
• can be used in less accessible organs
Cons:
• limited information about gene product (mRNA,
protein etc)
• needs cloning and transformation
• neglects regulatory elements (introns, UTRs
etc.)
• length of promoter given arbitrarily
Translational GFP fusions
your genepromoter
here can
be GFP
here can
be GFP
terminator
your genepromoter terminator
your genepromoter terminator
here can
be GFP
N-terminal fusion
C-terminal fusion
fusion inside the coding sequence
GFP and membrane proteins
here can
be GFP
It is good to
have GFP tag
localized inside
the cell (plants)
Expression of isoforms
cDNA1
cDNA2
YFP
YFP
Kriechenbaumer et al 2011Not the best option available – can you guess?
endoplasmic
reticulum
cytosol
Isn’t this better?
YFP
GFP
Expression of isoforms
Fluorescent protein fusion
Pros:
•
Cons:
Fluorescent protein fusion
Pros:
• in vivo imaging
Cons:
• not always functional
• transformation needed
• transparent material (you can sometimes fix
GFP signal, however)
• sometimes GFP artifacts (tag doesn’t allow
proper targeting)
Why to visualize all this stuff
pSHR :: GFP pSHR::SHR::GFP
Nakajima et al, Nature 2001
promoter translational
Why to visualize all this stuff
pSHR :: GFP pSHR::SHR::GFP
1 2 3 1 2 3
1 – epidermis
2 – cortex
3 – endodermis
4 – stele
promoter translational
44
Why to visualize all this stuff
pSHR :: GFP pSHR::SHR::GFP
Nakajima et al, Nature 2001
BANG! SHR moves from stele to endodermis
Protein immunolocalization
(of given source
organism)
Most favorite animals:
-rabbit (too many rabbits)
-mouse (low volume)
-goat
-chicken
-rat
-sheep
-donkey
-guinea pig
2ndary: antirabbit from no-rabbit, antimouse from
no-mouse, etc.
Protein immunolocalization
immunolocalization - fluorescently
fluorescent
dye attached
primary
antibodies
secondary
antibodies
Protein immunolocalization
immunolocalization
• FITC (obsolete)
• CY3, CY5
• Alexa (488, 568, 633)
Fluorescent dyes conjugated
to 2ndary (examples):
www.zeiss.com/microscopy
Protein immunolocalization
Pros:
•
•
Cons:
•
•
Protein immunolocalization
Pros:
• no need to clone or transform or cross
• direct (if no tag used)
• allows sectioning (less accessible tissues)
Cons:
• fixed material only
• excellent antibodies only, sometimes tricky
GFP tag partially retains PIN1 in
endoplasmic reticulum (-> artifact)
PIN1-GFP anti-PIN1
Protein localization - immunogold
immunolocalization - immunogold
electron microscope
Immunogold collocalization
Nopp140 (5 nm gold particles)
nascent DNA (10 nm)
Philimonenko et al 2000, and an unfortunate Cell paper
Pros/cons
Pros:
• direct
• nothing can beat the resolution
Cons:
• very tricky (needs rather expert)
• huge experience for interpretation needed
Can we visualize postranslational
modifications?
Also RNA can be
visualized
Localization of mRNA
RNA hybridization in situ
Visualization of mRNA
RNA hybridization in situ
Pros
• classical technique in developmental biology
• no transgenes needed
Cons
• tedious, tricky, no success guaranteed
• only on fixed samples
For shorter RNAs (miRNA etc.):
• LNA probes needed
Also mRNA can be
visualized in vivo
Ash1 mRNA localized to the tip of the daughter cell
λN22 system – RNA imaging
in vivo
nuclear localization signal
promoter
viral RNA
binding
protein
Drawbacks of λN22 system
- we have SPINACH
GACGCAACUGAAUGAAA
UGGUGAAGGACGGGUCC
AGGUGUGGCUGCUUCGG
CAGUGCAGCUUGUUGAG
UAGAGUGUGAGCUCCGU
AACUAGUCGCGUC
+
Paige et al. 2012
RNA fusion aptamer
blue-DNA green-RNA
Other vegetables than SPINACH
Paige et al. 2012; Song et al. 2014
Advanced confocal techniques
(slightly) Advanced confocal
techniques
• FRAP
• photoactivatable FP
• FCS
FRAP
region of interest (ROI)
Fluorescence Recovery After Photobleaching
FRAP
you can quantify fluorescence..
(ImageJ is our friend)
mean min max
A 90.404 49 113
C 8.556 3 8
D 39.934 19 63
FRAP – bleaching curve
What does the curve tell?
FRAP – bleaching curve
iFRAP
inverse FRAP
iFRAP – dissociation of
premRNA from specles
FRAP derivatives
FLIP
Fluorescence Loss After Photobleaching
• bleaching process is repeated during the experiment
• for studying general protein turnovers in compartments
• is there a fraction of protein which does not leave the bright
green patches?
continuous bleaching here
FRAP derivatives
FLAP
Fluorescence Localization after Photobleaching
• two fluorochromes on one protein– one bleached, non
bleached as control
Perhaps better scheme than
previous
YFP bleachedCFP not bleached
prebleach after bleach RED=CFP-YFP
Dunn et al. 2002
FRAP - advantages
• not only proteins (also other dyes)
• tells you more than simple life imaging
movie
• your cells are moving
• high energy needed to bleach the ROI
– long time needed to bleach
– can damage your material
• usually only one ROI can be observed –
time consuming
• for gourmets perhaps awkward (although
more reliable and robust)
FRAP – pitfalls
aquaporin PIP2
undergoes
lateral difussion
photoactivation
(UV)
Photoactivable
fluorescent proteins
Photoactivable proteins
Dronpa, Kaede, Eos – probably most popular
Photoactivable proteins
Advantages:
-elegant, can be convincing
Disadvantages:
-very weak signal
-each material needs optimization
Remarks
• your material is 3D
• protein de novo synthesis in some
experiments (e.g. cycloheximide stops
translation)
FLIM
Fluorescence Life Time Imaging Microscopy
Fluorochromes
• excitation spectra
• emission spectra
• unique lifetime
FLIM - applications
FLIM - applications
Protein-protein interactions
(FRET-FLIM) (other lecture)
Lifetime sensitive to almost everything:
• pH
• ionic strength
• solution polarity
• other fluorochrome
FLIM
Trautmann et al. PicoQuant Application note 2013
indeed, salt changes fluorophore life time
(American cockroach glands)
FLIM - discrimination of
autofluorescence
Q: What is easier
experiment to confirm
autofluorescence?
Dovzhenko, TrautmannPicoQuant Application note 2013
(be careful with the interpretation)
FLIM
• need to have experience
• need to have special module on your
confocal
FCS
Fluorescence Correlation Spectroscopy
t + τ It is counted,
how many times
the fluorescent
molecule comes
through the
focal plane.
autocorrelation analysis
Autocorrelation
analysis: the
way how to
discriminate the
diffusions
speeds of
particles.
FCS
Schwille und Haustein
 [ms]
G()
antibunching
rotational movement
photophysical process
(triplet state, …)
diffusion
FCS (FCCS)
fluorescence cross-correlation spectroscopy
Digman and Gratton 2011
Literature
• Paige et al., RNA Mimics of Green Fluorescent Protein, Science 333, 642-646, 2011 (SPINACH
and other vegetables)
• https://www.micro-shop.zeiss.com/index.php?s=452278238ae52c&l=en&p=de&f=f&a=d
(comprehensive and broad list of phluorochromes)
• http://www.illuminatedcell.com/ - nicely done pages about plant cell imaging
• Ishikawa-Ankerhold et. al. Advanced Fluorescence Microscopy Techniques — FRAP, FLIP,
FLAP, FRET and FLIM, Molecules 2012, 17, 4047-4132
• Sambrook & Russell Molecular Cloning: A Laboratory Manual, Third Edition, Cold Spring Harbor
Laboratory Press; 3rd edition (January 15, 2001), 13.5 pounds weight
• Ctirad Hofr – Pokročilé biofyzikální metody v experimentální biologii (přednáška)
Photon bunching,
if someone would ask