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 NALIN NAYAN
 OPTOMETRIST
 It is a medical imaging technique used to visualize the
inside of blood vessels and organs of the body, with
particular interest in the arteries, veins and the heart
chambers.
 traditionally done by injecting a radio-opaque contrast
agent into the blood vessel and imaging using X-ray
based techniques
 The word itself comes from the Greek words angeion,
"vessel", and graphein, "to write or record".
 The film or image of the blood vessels is called an
angiograph, or more commonly, an angiogram.
- Fundus Fluorescein angiography refers
to photographing fluroscein dye in the
retinal vasculature following intravenous
injection of fluroscein sodium.
- Described in 1959 by MacLean and
Maumenee
 Fluorescein (C20H12O5)
refers to Fluorescein
sodium (C20H10Na2).
 Is a brown or orange-red
crystalline substance first
synthesized in 1871 in
Germany by Von Baeyer
 1882 – Ehrlich introduced Fluorescein into
investigative ophthalmology
 1940 – Gifford studied aqueous dynamics after
injecting intravenous Fluorescein
 1960 – 2 medical students Novotny & Alwis
experimented on each other and developed
FFA
 Non toxic, inexpensive, safe
 Alkaline solution
 Highly fluorescent
 Absorbs blue light (480-500 nm)
 Emits yellow-green (500-600 nm [525
nm])
 Effective at pH 7.37-7.45
 Removal from blood by kidneys and liver
within 5 hrs.
 Inner and Outer blood retinal barriers
control movement of fluid, ions &
electrolytes from intravascular space to
extracellular space in retina
 FFA – method of examining competence
of blood retinal barriers and making
permanent record
 GENERAL PRINCIPLES:-
-Fluorescein binding.
-Inner blood retinal barrier.
-Major choroidal vessels.
-Outer blood retinal barrier.
-Excitation peak.
-Types of filters.
 70-85% fluorescein molecules bind to
serum proteins (mainly albumin) on
entering the circulation.
 The rest unbound molecules are referred
to as free fluorescein.
 At level of retinal capillary endothelium (tight
junctions, non-fenestrated) and basement
membrane
 Prevents all leaks of free fluorescein and
albumin-bound fluorescein.
 in vascular permeability caused by changes in
intravascular pressure or tissue hydrostatic
pressure, or by change in capillary walls
themselves, will permit leakage of both bound &
free fluorescein molecules in extra vascular
space.
-impermeable to both bound & free
fluorescein molecules.
- walls of choricapillaries are extremely
thin & contain multiple fenestrations
through which free fluorescein molecules
are able to escape into the extra vascular
space & across Bruch’s membrane.
 Composed of intact RPE (tight junctions
b/w RPE cells).
 Impermeable to free fluorescein.
 RPE presents an optical barrier to
fluorescein and masks choroidal
circulation
 490 nm (blue part of spectrum).
 represents maximal absorption of light
energy by fluorescein.
 Molecules stimulated by this wavelength
will be excited to higher energy level &
will emit light of longer wavelength
( green portion of spectrum i.e. at 530 nm
).
 2 types of filters:-
- cobalt-blue excitation.
- yellow-green barrier.
Ensures blue light enters the eye & only
yellow green light enters the camera.
 Light emitted from retinal camera passes
through blue excitation filter, emerging
blue light enters the eye & excites
Fluorescein molecules in retinal & choroid
circulation of longer wavelength (yellow
green).
 Yellow green barrier filter thus blocks any
blue light that may leave eye, allowing only
yellow-green light to pass through
unimpaired to be recorded on film.
- Pupil should be dilated.
TECHNIQUE:-
- Patient seated in front of camera with one arm
out stretched.
- Fluorescein 5 ml of 10% solution is drawn up
into syringe.
In opaque media, 3 ml of 25% solution may be
preferred, because it gives better result.
- Red free photograph is taken.
- Fluorescein injected rapidly into antecubital
vein.
- Photographs are taken at approx 1 sec interval
between 5 & 25 sec after injection.
- After transit phase has been photographed in
eye, control pictures are taken of opposite eye.
If necessary, late photograph can also be
taken after 10 min & occasionally after 20 min if
leakage is anticipated.
 Red after image.
 Transient nausea.
 Flushing of skin.
 Itching.
 Hives.
 Excessive sneezing.
 Discolouration of urine & skin.
 Baseline photos and red free
 5 Phases of FFA
 Choroidal phase
 Arterial phase
 Capillary phase
 Venous phase
 Late phase
1) CHOROIDAL OR PRE-ARTERIAL PHASE:-
-Choroidal circulation is filling, but no dye has
reached the retinal arteries.
2) ARTERIAL PHASE:-
-follows 1 sec after pre-arterial phase.
-extends from first appearance of dye in the
arteries until whole arterial circulation is filled.
3)CAPILLARY OR ARTERIOVENOUS PHASE:-
-characterized by complete filling of the arteries
& capillaries with early lamellar flow in the
veins.
4) VENOUS PHASE:-
- subdivided into early, mid & late stages according to
extent of venous filling & arterial emptying.
early venous phase:- shows complete arterial & capillary
filling, & lamellar venous flow.
mid venous phase:- shows almost complete venous filling.
late venous phase:- shows complete venous filling.
-arteries are beginning to show decreasing
fluorescence.
-Recirculation of dye occurs within 3-5 min.
-The intensity of fluorescence begins to diminish so
that arteries & veins appear equally fluorescent.
5) LATE PHASES:-
- shows effects of continuous recirculation,
dilution & elimination of dye.
- with each succeeding wave, the intensity
of fluorescence becomes weaker.
- late staining of optic nerve is a normal
finding.
 Arm to retina (ONH) 7-12s
 Posterior- ciliary artery fill 9s
 Choroidal flush, cilio-retinal artery 10s
 Retinal arterial phase 10-12s
 Capillary transition phase 13s
 Early venous/lamellar/a-v phase 14-15s
 Venous phase 16-17s
 Late venous phase 18-20s
 Late phase 5 – 15 mins
12s arterial phase 15s early venous
20s venous phase 52s late phase
 Arterial phase may range from 2-30s;
 may be affected by:
- cardiac disease
- blood viscosity
- vessel calibre
- CCF
- GCA
- BP↑
- carotid artery stenosis.
 Superior arterioles fill before inferior and
temporal before nasal
 Choroidal & scleral fluorescence depends on
pigment density of RPE & its integrity
 Macular hypo fluorescence – due to ’d density↑
of RPE & xanthophyll blocking choroidal
fluorescence
 No retinal capillaries – FAZ 500μm; foveola
350μm
 Only 2 fundamental principles in FFA
- HYPER fluorescence or
HYPO fluorescence !
 MAY BE CAUSED BY:-
1) AN RPE WINDOW DEFECT:
-RESULTING FROM ATROPHY OF
OVERLYING RPE CELLS WITH
UNMASKING OF NORMAL
BACKGROUND CHOROIDAL
FLUORESCENCE.
2) POOLING OF DYE:-
-UNDER A DETACHMENT OF RPE OR IN
IN THE SUB RETINAL SPACE.
- CAUSED BY A BREAKDOWN OF
OUTER BLOOD RETINAL BARRIER.
3) LEAKAGE OF DYE:-
- into the sensory retina as a result of
breakdown of inner blood retinal barrier.
- may be:-
~from choroidal new vessels.
~from retinal new vessels.
~from the optic nerve head
(in papilloedema).
4) STAINING OF TISSUES:-
- as a result of prolonged retention of
fluorescence.
 Permeability defects cause pooling &
staining
 Pooling – serous RPE detachment, SRF (↑
in size, shape & intensity in later phases)
 Staining – sclera, ON, drusen, vasculitis.
(Leak into tissue rather than anatomical space)
 May be caused by :-
1) BLOCKAGE OF FLUORESCENCE:-
- by increased density of pigment
(xanthophyll -sensory retina,
melanin- RPE)
- deposition of abnormal materials
( hard exudates in sensory retina,
lipofuscin in Best’s disease)
- Blood.
2)obstruction of retinal and choroidal
circulation:-
- preventing access of fluorescein to the
tissues.
3) loss of vascular tissues:-
- in severe myopic degeneration or
choroideremia.
 Due to the 2 barrier filters not having
mutually exclusive transmission spectra
 Light from bright fundal structures can
pass through both filters & expose film.
e.g. ONH drusen, astrocytic hamartomas
 Autofluorescence can
be diagnostic
 FFA can exclude
papilloedema
 Saves pt from
invasive neuro
diagnostic
procedures!
Optic nerve head drusen
 CB readily leaks fluorescein during
aqueous production, into ocular fluids.
 Green light emitted when excited by
blue light. Illuminates light coloured
structures eg: MNF’s, white lesions
 To aid diagnosis
 Decisions on whether to Rx or not
 Always study FFA’s with other relevant
investigations before making final
diagnosis
 Start by describing obvious abnormality
 Describe hypo/hyperfluorescent
components
 Intensity of fluorescence with time
 Area of fluorescence & changes with time
 Run through anatomical list describing
any other abnormalities affecting
structures below:
 Macula
 Disc
 Major arcades
 Capillaries
 Early venous phase
 HyperF – NVD, ma’s
 HypoF – blocked due
to blood
 HypoF retinal
haem 1 ischaemia 2
 HyperF ma’s 3, nv’s 4
 IRMA 5
 Venous beading 6
 HyperF – ma’s (leak)
& laser spots (stain)
 HypoF – pigmented
scars, blood,
capillary drop out
 HypoF – massive
retinal capillary
dropout, pigmented
laser scars
 HyperF – laser scar
staining
 HypoF – retinal
capillary closure, SRF,
blood
 HyperF – retinal vein
damage – staining
collagen, leaking
through damaged
endothelial walls
 HyperF – damaged
veins staining and
leaking, ma’s
 HypoF – subretinal
and preretinal haems
 Collaterals don’t
leak!
 Non-perfusion of retinal
vasculature.Vessels appear
dark against light background
 No capillary perfusion, so
empty veins (cattle-trucking)
 Choroidal perfusion intact
(hence “cherry red spot”); C-
R artery sparing in 15%
 RPE atrophy allows
choroidal fluorescence
through with choroidal
“flush”
 Does not change size or
shape with time
 Fades with choroidal
fluorescence
Red Free
Late
 Large area of GA
 Clear view of
choroidal vessels
 FFA shows
unmasking of
choroidal vessels
 RPE “show-through”
 Loss of masking
 Early lighting up with
choroid
 Small defect in outer
BR barrier
 F enters RPE defect &
fills serous retinal
elevation “blister” (7%
cases)
 HyperF - ’s in size &↑
intensity
Early
Late
 Breakdown of internal BR
barrier
 Early leak from
parafoveal retinal vessels
– hyperF, in FAZ↓
 Late pooling in classic
“petalloid” appearance
(NFL)
 Ischaemia & vasculitis
incompetent endothelial
TJ’s
 F leaks into CT of bv’s &
stains it.This persists
 Late disc staining is
normal
ARN
Pars planitis
 Early lacey hyperF
“classic”
 HypoF “halo” – blood
&/or macula pigment
 Late leak, blurred
margins & apparent ↑
in size
 Type I – PED – well-
defined area of early
hyperF, margins
unchanged
 Type II – late leak of
undeyermined
source – not obvious
from early phase
Choroidal naevus blocking choroidal fluorescence in arterial phase
 Stargardt’s – “dark
choroid” (early)
 Lipofuscin deposition
at RPE
 Fluorescein Angiography, technique
interpretation & application, Max
Nanjiani (OMP)
 www.mrcophth.com/ffainterpretation

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BASIC INFO ON FUDUS FLORESCENCE ANGIOGRAPHY

  • 1.  NALIN NAYAN  OPTOMETRIST
  • 2.  It is a medical imaging technique used to visualize the inside of blood vessels and organs of the body, with particular interest in the arteries, veins and the heart chambers.  traditionally done by injecting a radio-opaque contrast agent into the blood vessel and imaging using X-ray based techniques  The word itself comes from the Greek words angeion, "vessel", and graphein, "to write or record".  The film or image of the blood vessels is called an angiograph, or more commonly, an angiogram.
  • 3. - Fundus Fluorescein angiography refers to photographing fluroscein dye in the retinal vasculature following intravenous injection of fluroscein sodium. - Described in 1959 by MacLean and Maumenee
  • 4.  Fluorescein (C20H12O5) refers to Fluorescein sodium (C20H10Na2).  Is a brown or orange-red crystalline substance first synthesized in 1871 in Germany by Von Baeyer
  • 5.  1882 – Ehrlich introduced Fluorescein into investigative ophthalmology  1940 – Gifford studied aqueous dynamics after injecting intravenous Fluorescein  1960 – 2 medical students Novotny & Alwis experimented on each other and developed FFA
  • 6.  Non toxic, inexpensive, safe  Alkaline solution  Highly fluorescent  Absorbs blue light (480-500 nm)  Emits yellow-green (500-600 nm [525 nm])  Effective at pH 7.37-7.45  Removal from blood by kidneys and liver within 5 hrs.
  • 7.  Inner and Outer blood retinal barriers control movement of fluid, ions & electrolytes from intravascular space to extracellular space in retina  FFA – method of examining competence of blood retinal barriers and making permanent record
  • 8.  GENERAL PRINCIPLES:- -Fluorescein binding. -Inner blood retinal barrier. -Major choroidal vessels. -Outer blood retinal barrier. -Excitation peak. -Types of filters.
  • 9.  70-85% fluorescein molecules bind to serum proteins (mainly albumin) on entering the circulation.  The rest unbound molecules are referred to as free fluorescein.
  • 10.  At level of retinal capillary endothelium (tight junctions, non-fenestrated) and basement membrane  Prevents all leaks of free fluorescein and albumin-bound fluorescein.  in vascular permeability caused by changes in intravascular pressure or tissue hydrostatic pressure, or by change in capillary walls themselves, will permit leakage of both bound & free fluorescein molecules in extra vascular space.
  • 11. -impermeable to both bound & free fluorescein molecules. - walls of choricapillaries are extremely thin & contain multiple fenestrations through which free fluorescein molecules are able to escape into the extra vascular space & across Bruch’s membrane.
  • 12.  Composed of intact RPE (tight junctions b/w RPE cells).  Impermeable to free fluorescein.  RPE presents an optical barrier to fluorescein and masks choroidal circulation
  • 13.  490 nm (blue part of spectrum).  represents maximal absorption of light energy by fluorescein.  Molecules stimulated by this wavelength will be excited to higher energy level & will emit light of longer wavelength ( green portion of spectrum i.e. at 530 nm ).
  • 14.  2 types of filters:- - cobalt-blue excitation. - yellow-green barrier. Ensures blue light enters the eye & only yellow green light enters the camera.
  • 15.  Light emitted from retinal camera passes through blue excitation filter, emerging blue light enters the eye & excites Fluorescein molecules in retinal & choroid circulation of longer wavelength (yellow green).  Yellow green barrier filter thus blocks any blue light that may leave eye, allowing only yellow-green light to pass through unimpaired to be recorded on film.
  • 16. - Pupil should be dilated. TECHNIQUE:- - Patient seated in front of camera with one arm out stretched. - Fluorescein 5 ml of 10% solution is drawn up into syringe. In opaque media, 3 ml of 25% solution may be preferred, because it gives better result.
  • 17. - Red free photograph is taken. - Fluorescein injected rapidly into antecubital vein. - Photographs are taken at approx 1 sec interval between 5 & 25 sec after injection. - After transit phase has been photographed in eye, control pictures are taken of opposite eye. If necessary, late photograph can also be taken after 10 min & occasionally after 20 min if leakage is anticipated.
  • 18.  Red after image.  Transient nausea.  Flushing of skin.  Itching.  Hives.  Excessive sneezing.  Discolouration of urine & skin.
  • 19.  Baseline photos and red free  5 Phases of FFA  Choroidal phase  Arterial phase  Capillary phase  Venous phase  Late phase
  • 20. 1) CHOROIDAL OR PRE-ARTERIAL PHASE:- -Choroidal circulation is filling, but no dye has reached the retinal arteries. 2) ARTERIAL PHASE:- -follows 1 sec after pre-arterial phase. -extends from first appearance of dye in the arteries until whole arterial circulation is filled. 3)CAPILLARY OR ARTERIOVENOUS PHASE:- -characterized by complete filling of the arteries & capillaries with early lamellar flow in the veins.
  • 21. 4) VENOUS PHASE:- - subdivided into early, mid & late stages according to extent of venous filling & arterial emptying. early venous phase:- shows complete arterial & capillary filling, & lamellar venous flow. mid venous phase:- shows almost complete venous filling. late venous phase:- shows complete venous filling. -arteries are beginning to show decreasing fluorescence. -Recirculation of dye occurs within 3-5 min. -The intensity of fluorescence begins to diminish so that arteries & veins appear equally fluorescent.
  • 22. 5) LATE PHASES:- - shows effects of continuous recirculation, dilution & elimination of dye. - with each succeeding wave, the intensity of fluorescence becomes weaker. - late staining of optic nerve is a normal finding.
  • 23.  Arm to retina (ONH) 7-12s  Posterior- ciliary artery fill 9s  Choroidal flush, cilio-retinal artery 10s  Retinal arterial phase 10-12s  Capillary transition phase 13s  Early venous/lamellar/a-v phase 14-15s  Venous phase 16-17s  Late venous phase 18-20s  Late phase 5 – 15 mins
  • 24. 12s arterial phase 15s early venous 20s venous phase 52s late phase
  • 25.  Arterial phase may range from 2-30s;  may be affected by: - cardiac disease - blood viscosity - vessel calibre - CCF - GCA - BP↑ - carotid artery stenosis.
  • 26.  Superior arterioles fill before inferior and temporal before nasal  Choroidal & scleral fluorescence depends on pigment density of RPE & its integrity  Macular hypo fluorescence – due to ’d density↑ of RPE & xanthophyll blocking choroidal fluorescence  No retinal capillaries – FAZ 500μm; foveola 350μm
  • 27.  Only 2 fundamental principles in FFA - HYPER fluorescence or HYPO fluorescence !
  • 28.  MAY BE CAUSED BY:- 1) AN RPE WINDOW DEFECT: -RESULTING FROM ATROPHY OF OVERLYING RPE CELLS WITH UNMASKING OF NORMAL BACKGROUND CHOROIDAL FLUORESCENCE.
  • 29. 2) POOLING OF DYE:- -UNDER A DETACHMENT OF RPE OR IN IN THE SUB RETINAL SPACE. - CAUSED BY A BREAKDOWN OF OUTER BLOOD RETINAL BARRIER.
  • 30. 3) LEAKAGE OF DYE:- - into the sensory retina as a result of breakdown of inner blood retinal barrier. - may be:- ~from choroidal new vessels. ~from retinal new vessels. ~from the optic nerve head (in papilloedema).
  • 31. 4) STAINING OF TISSUES:- - as a result of prolonged retention of fluorescence.
  • 32.  Permeability defects cause pooling & staining  Pooling – serous RPE detachment, SRF (↑ in size, shape & intensity in later phases)  Staining – sclera, ON, drusen, vasculitis. (Leak into tissue rather than anatomical space)
  • 33.  May be caused by :- 1) BLOCKAGE OF FLUORESCENCE:- - by increased density of pigment (xanthophyll -sensory retina, melanin- RPE) - deposition of abnormal materials ( hard exudates in sensory retina, lipofuscin in Best’s disease) - Blood.
  • 34. 2)obstruction of retinal and choroidal circulation:- - preventing access of fluorescein to the tissues. 3) loss of vascular tissues:- - in severe myopic degeneration or choroideremia.
  • 35.  Due to the 2 barrier filters not having mutually exclusive transmission spectra  Light from bright fundal structures can pass through both filters & expose film. e.g. ONH drusen, astrocytic hamartomas
  • 36.  Autofluorescence can be diagnostic  FFA can exclude papilloedema  Saves pt from invasive neuro diagnostic procedures! Optic nerve head drusen
  • 37.  CB readily leaks fluorescein during aqueous production, into ocular fluids.  Green light emitted when excited by blue light. Illuminates light coloured structures eg: MNF’s, white lesions
  • 38.  To aid diagnosis  Decisions on whether to Rx or not  Always study FFA’s with other relevant investigations before making final diagnosis
  • 39.  Start by describing obvious abnormality  Describe hypo/hyperfluorescent components  Intensity of fluorescence with time  Area of fluorescence & changes with time
  • 40.  Run through anatomical list describing any other abnormalities affecting structures below:  Macula  Disc  Major arcades  Capillaries
  • 41.  Early venous phase  HyperF – NVD, ma’s  HypoF – blocked due to blood
  • 42.  HypoF retinal haem 1 ischaemia 2  HyperF ma’s 3, nv’s 4  IRMA 5  Venous beading 6
  • 43.  HyperF – ma’s (leak) & laser spots (stain)  HypoF – pigmented scars, blood, capillary drop out
  • 44.  HypoF – massive retinal capillary dropout, pigmented laser scars  HyperF – laser scar staining
  • 45.  HypoF – retinal capillary closure, SRF, blood  HyperF – retinal vein damage – staining collagen, leaking through damaged endothelial walls
  • 46.  HyperF – damaged veins staining and leaking, ma’s  HypoF – subretinal and preretinal haems
  • 48.  Non-perfusion of retinal vasculature.Vessels appear dark against light background  No capillary perfusion, so empty veins (cattle-trucking)  Choroidal perfusion intact (hence “cherry red spot”); C- R artery sparing in 15%
  • 49.  RPE atrophy allows choroidal fluorescence through with choroidal “flush”  Does not change size or shape with time  Fades with choroidal fluorescence Red Free Late
  • 50.  Large area of GA  Clear view of choroidal vessels  FFA shows unmasking of choroidal vessels
  • 51.  RPE “show-through”  Loss of masking  Early lighting up with choroid
  • 52.  Small defect in outer BR barrier  F enters RPE defect & fills serous retinal elevation “blister” (7% cases)  HyperF - ’s in size &↑ intensity Early Late
  • 53.  Breakdown of internal BR barrier  Early leak from parafoveal retinal vessels – hyperF, in FAZ↓  Late pooling in classic “petalloid” appearance (NFL)
  • 54.  Ischaemia & vasculitis incompetent endothelial TJ’s  F leaks into CT of bv’s & stains it.This persists  Late disc staining is normal ARN Pars planitis
  • 55.  Early lacey hyperF “classic”  HypoF “halo” – blood &/or macula pigment  Late leak, blurred margins & apparent ↑ in size
  • 56.  Type I – PED – well- defined area of early hyperF, margins unchanged  Type II – late leak of undeyermined source – not obvious from early phase
  • 57. Choroidal naevus blocking choroidal fluorescence in arterial phase
  • 58.  Stargardt’s – “dark choroid” (early)  Lipofuscin deposition at RPE
  • 59.  Fluorescein Angiography, technique interpretation & application, Max Nanjiani (OMP)  www.mrcophth.com/ffainterpretation