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Models of Mller Glial Cell Disruption and the Consequences on Retinal Health and
Visual Function in the Zebrafish Retina
NICOLAS A. YANNUZZIDepartment of Molecular and Cellular Biology, Harvard University,
Cambridge, Massachusetts 02138
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Statement of ResearchThis thesis was completed under the guidance of Dr. Pamela M. Kainz and Dr.
John E. Dowling at the Department of Molecular and Cellular Biology at Harvard
College. Research was conducted from September, 2005 - May, 2006 and from
September, 2006 - April, 2007.
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ACKNOWLEDGEMENTS
I began working at the Dowling Lab with the intention of completing my single
semester research requirement. Within a short time, however, I found that the
opportunity to conduct my own research was not only a privilege, but also a chance for
me to witness the active pursuit of scientific discovery. The completion of this thesis was
the most meaningful, enjoyable, and exciting part of my academic experience at Harvard.
It revived my love for science and research, and I am thankful for the freedom I was
given to express my thoughts and ideas during the project.
I would like to thank Dr. Pamela Kainz for all of her help and support during the
process and for teaching me everything I know about scientific research, from
experimental design to thoughtful data interpretation. Dr. Kainz is not only a great
scientist, but also a great teacher. I would also like to thank the other members of the
Dowling Lab for helping me during the process. Finally, I would like to thank my
mother for her support and my father for instilling in me a passion for scientific thought
and discovery. His achievements in ophthalmology inspired me to pursue research on the
retina.
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ABSTRACT
Mller cells are the primary glial cells of the vertebrate retina. They contact and ensheath
every retinal cell type and regulate neuronal activity. Recent studies have suggested that
Mller cells also provide specific supportive roles for the survival and function of
photoreceptor cells, but there are currently few models where this relationship can beexplored. The purpose of this study was to evaluate two candidate models of Mller cell
disruption and to observe the consequences on retinal health and visual function. In the
first chapter I investigated a potential pharmacological model of Mller cell stress. Usingthe gliotoxin -aminoadipic acid (-AAA), I observed only a modest sign of Mller cell
stress in adult zebrafish, while the effect on larvae was not glial-specific indicated by the
presence of pyknotic nuclei among retinal neurons. Since -AAA failed to produce clearand reproducible signs of glial cell defects, I decided to discontinue my pursuit of this
model and instead investigate a potential genetic model of Mller cell disruption by
characterizing the rose mutant, an endothelin receptor B (ET-B) gene knockout. I foundthat the morphology of the larval rose retina appeared normal. However, when exposed
to constant light, wild type larvae were unaffected while the rose larval retina sufferedrod outer segment disruption, loss of 10% of the cells in the inner nuclear layer, where
the Mller cell bodies lie, and a decrease in visual sensitivity. These defects areconsistent with the hypothesis that compromised Mller glial cells lead to a decrease in
photoreceptor cell resilience. Questions remain as to what extent Mller cells are
involved in the light exposed rose phenotype, but this study provides the groundwork forcontinued exploration concerning how the absence of ET-B compromises the retina and
the ways Mller cells may be involved in the preservation of photoreceptor cells.
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GENERAL INTRODUCTION
Glial cells provide physical support and protection for neurons and guide
migrating neurons to their destinations in the brain during development. Glia have also
been shown to act as a template for axonal migration in the neural retina (Silver and
Rutishauser, 1984). Furthermore, they regulate the formation of synapses that enable
neuronal correspondence and promote the survival of some neurons while playing a role
in the birth of others (Helmuth, 2001).
Once dismissed by neuroscientists as playing a minimal role in the nervous
system, glia have recently been suspected to be involved significantly in the pathogenesis
of certain diseases. Research has shown that glia are integral to the understanding and
causes of neuropathic pain, epilepsy, and neurodegenerative diseases (Miller, 2005).
Studies have also suggested that glia may offer a new range of therapeutic targets in a
variety of diseases including Multiple Sclerosis and some psychiatric disorders, where
post mortem studies have demonstrated that there are abnormal amounts of glia in certain
areas of the brain (Miller, 2005).
Research on glia has not been limited to their function in the brain, where they
outnumber neurons in a ratio of ten to one. Glia have also been studied in the context of
the vertebrate retina. Mller glia are the primary support cells in the retina. They contact
and ensheath every retinal cell type and regulate neuronal activity by controlling
extracellular ion concentration and by recycling excess neurotransmitters used during
signaling processes (Newman and Reichenbach, 1996; Sarthy and Ripps, 2001).
Specifically, they express gated channels and neurotransmitter receptors which can cause
depolarization and intracellular Ca2+
waves. In addition, they transport K+
and glutamate
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and regulate retinal pH levels via carbonic anhydrase (Newman and Reichenbach, 1996).
Although there are more neurons than Mller cells, Mller cell processes contact and
ensheath the synaptic and nuclear region of every cell in the retina; their nuclei reside in
the inner nuclear layer, which also contains horizontal, amacrine and bipolar cell nuclei,
and their endfeet project from the ganglion cell layer (Fig. 1), allowing for extensions that
span the entire depth of the neural retina (Peterson et al., 2001). Their apical processes
also contact the inner segments of photoreceptors. This framework provides a basis for
interaction with every neuron.
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Fig. 1. The various layers of the retina are labeled for convenience (Source: The purple and white illustration, exceptfor the illustration of the Mller cell (right) and the photograph of the adult zebrafish retina (left), is courtesy of TheWashington University School of Medicine). Mller cells and their processes span the width of the neural retina.Their cell bodies reside in the inner nuclear layer, and their endfeet project out of the ganglion cell layer, while their
apical processes reach the outer segments. Rod outer segments are also labeled and are located directly under thepigment epithelium.
MllerCellBody
MllerEndfeet
ApicalProcesses
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Both clinical and scientific investigators have suggested that Mller cells play a
vital role in several retinal diseases such as X-linked Retinoschisis (Reid et al., 1999),
Cystoid Macular Degeneration (Loeffler et al., 1992), Idiopathic Macular Holes, and
Foveomacular Schisis (Gass, 1999). There has even been some suspicion that Mller cell
disease may be a principal agent in certain forms of Age Related Macular Degeneration,
the leading cause of blindness (DiLoreto et al., 1995). Clinical researchers suggest that
Mller cells are not necessarily a cause of disease. Instead, they believe that Mller cells
become reactive and hypertrophic in response to photoreceptor damage and eventually
lead to scarring. Because the activation of Mller cells in response to preexisting
problems with the neural retina is so common, it has been the main focus in the research
of retinal glia.
Virtually no clinical studies and very few animal studies have explored how
Mller cells themselves could be the primary cause of failing retinal health or function
and not just a response to preexisting damage. Thus, while some of the functions of
Mller cells have been determined, the precise relationship between Mller cells and
retinal cell health and maintenance is not yet fully understood. The effect of Mller cell
disruption on photoreceptor cells was the specific relationship that I set out to explore in
this study. The discovery that stressing or eliminating Mller cells could lead to
photoreceptor degeneration (DiLoreto et al., 1995) provided in part, the inspiration for
this thesis.
The chosen model organism for studying the relationship between retinal glia and
neurons was the zebrafish. Zebrafish are small, approximately one inch long freshwater
fish that can be raised inexpensively and in large numbers. Embryos develop rapidly
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resulting in zebrafish eyes that exhibit light response in just 3 days post fertilization (dpf)
(Brokerhoff et al., 1995). The zebrafish retina has the same cell classes and architecture
as other vertebrates, including humans. However, unlike the mammalian retina, which
contains astrocytes, the zebrafish retina contains only Mller glia and sparse microglia.
An advantage of using the larval zebrafish is that it lacks scales; therefore, the absorption
of a drug can occur readily through its skin. Finally, the visual behavior of larvae can be
tested using the optokinetic response assay (OKR), in which their eyes track the
movement of vertical black and white stripes passing through their visual field. This
response is not only common to zebrafish but to all vertebrates. Using this assay, their
visual threshold can be quantified by determining the lowest level of light at which their
eyes consistently track the moving stripes.
The forefront of research concerning the role of Mller cells in the zebrafish
retina has focused on a genetic mutant called lazy eyes (lze). Larvae homozygous for the
lze mutation at 5 dpf respond much less robustly compared to wild type in the OKR
assay. Histological observations revealed that the mutation seemed to affect selectively
the Mller cells and photoreceptor cells. Some mutant retinas contained fewer Mller
cells than wild type retinas, while others contained Mller cells that appeared
hypertrophied or unhealthy. Most lze retinas had fewer rods and small cone outer
segments. The combined effects of light stress and genetic manipulation were also
studied, and constant light was found to accelerate drastically the Mller cell
degeneration and to accentuate the lze functional deficit (Kainz et al., 2003). The lze
mutant is thus a striking example of the special relationship between Mller cells and
photoreceptor cells. However, larvae homozygous for the lazy eyes mutation for some
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unknown reason die by 10 dpf. Therefore, there has yet to be a method of studying the
effects of Mller glial cell inactivity on the photoreceptor cells of the adult zebrafish
retina.
The overarching goal of my study was to explore two other potential models of
Mller cell disruption, one pharmacological and one genetic, and to determine if either of
these models resulted in compromised retinal health or function with special attention to
photoreceptors. For each model, photoreceptor stress, in the form of constant light, was
introduced and a morphological examination of the photoreceptors and Mller cells was
performed as well as an assessment of the function of the retina. In chapter one of this
thesis, I investigated a pharmacological model of Mller cell disruption by characterizing
the effects of the gliotoxin -aminoadipic acid (-AAA) on the wild type adult and larval
zebrafish. In chapter two, I examined a second potential model: a zebrafish mutant
missing the gene encoding endothelin receptor B (ET-B), which has been shown to be
expressed highly on Mller cells and involved in the response to light-induced stress on
photoreceptors (Rattner and Nathans, 2005).
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of zebrafish larvae. This delivery method was advantageous because the concentration of
the drug and the exposure time could be controlled precisely.
I monitored Mller stress both immunologically and histologically. Principally, I
followed the expression of antibodies for glial fibrillary acidic protein (GFAP) and
glutamine synthetase (GS), known Mller cell markers that have been shown to be
upregulated in times of retinal and Mller specific stress (Uhlmann et al., 2003). In
addition, I examined the histology of the adult and larval retinas for signs of Mller cell
hypertrophy and photoreceptor stress or death since I suspect that the health of these two
cell types is linked.
MATERIAL AND METHODS
Zebrafish maintenance
Wild type and lazy eyes heterozygous zebrafish were maintained in accordance to
Harvard University and National Institute of Health-approved protocols. The fish were
kept on a 14/10-hour light-dark cycle in 28.5C fish water containing 2g of Instant Ocean
salts per gallon of distilled water supplemented with vitamins. The lze mutant was
obtained from a family that had been isolated in a mutagenesis screen in which N-ethyl-
nitrosurea was used to induce DNA point mutations. The lze mutation is homozygous
recessive (Kainz et al., 2003).
Wild type larvae were obtained by mating several wild type fish together in a
basket cross. Lze larvae were obtained by mating adult fish heterozygous for the lze
mutation. The resultant progeny of this cross was comprised of wild type larvae, lze
mutants, and lze heterozygotes in a ratio of 1:1:2. Mutant lze were identified on 5 dpf
based on their failure to respond strongly in the OKR visual behavioral assay. Wild type
larvae repeatedly move their eyes with a smooth pursuit motion followed by a saccade in
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response to moving vertical black and white stripes. Mutant lze larvae respond with
weak and infrequent eye movements or fail completely to move their eyes (Kainz et al.,
2003). The adult zebrafish used in this experiment were genetically wild type and
approximately 30 months old.
Alpha-aminoadipic acid treatment of adult zebrafish and zebrafish larvae
DL--aminoadipic acid was mixed with PBS (pH 7.4) and then adjusted to a pH
of 7.3 using 1M NaOH. The resulting solution was mixed with fish water containing 2g
of Instant Ocean salts per gallon of distilled water supplemented with vitamins to various
concentrations.
Treated and untreated adult fish were kept in 400mL volume of liquid. Fish used
in experiments lasting longer than one day were fed once daily, and the water was
changed shortly after each feeding. Adult fish were exposed to concentrations of 1mM,
10mM, 25mM, and 50mM -AAA and for an incubation period from one to four days. It
has been suggested that adult fish absorb pharmacological agents into the blood stream
via the gills.
Treated and untreated larvae were kept in an incubator and were not fed
throughout the experiment because they still obtain nutrients from the yolk at this time in
development. Approximately 15-35 larvae were treated with 80mL of the toxin in a petri
dish starting at 3 dpf (after they had hatched from their chorion) and continuing for 48
hours until 5 dpf. The water was not changed after 3 dpf. Larvae were exposed to
concentrations of 10mM, 25mM, 50mM, and 100mM -AAA. Control larvae were
reared in normal fish water.
The larval exposure period of day 3 to day 5 was chosen for several reasons. On
the third day of life, retinal functions first begins in the zebrafish larvae, and on 5 dpf,
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visual function is readily observable and has been well-characterized (Schmitt and
Dowling, 1999; Brokerhoff et al., 1995). Another advantage to using young zebrafish
larvae for a pharmacological based experiment is that the larvae have not developed
scales yet and their skin is known to absorb chemicals in the fish water. Finally, based on
the work of Sugawara et al. on carp, exposure periods as short as 4-8 hours show
observable effects on Mller cells. Thus, a 48 hour exposure period was deemed a long
enough period of time.
Constant light rearing
Adult fish treated in constant light were first raised in constant darkness for one
week and were then placed in a box lined with several fluorescent bulbs, with a fan used
to minimize heat generated by the light for the duration of the treatment. The light level
was approximately 15,000 lux, about 50 times brighter than average room light, and the
temperature was maintained between 23-25C.
Preparation of adult eyes for immunohistology
Adult zebrafish were euthanized by over anesthetizing them in a 500mg/L
Tricaine solution and then decapitated. Adult heads were immediately placed into cold
fixative containing 4% paraformaldehyde (PFA) in 0.06M phosphate buffer, 3% sucrose
(pH 7.4) with 0.15mM CaCl2. Forceps were then used to loosen connective tissue
surrounding the eye, and the optic nerve was cut using a surgical scissor. Each eye was
removed gently and the cornea was poked with an insect pin to increase the access of the
fixative to the retina. Eyes were then transferred into fresh cold fixative and stored for 4-
8 hours at 4C. Eyes were washed for 5 minutes 3X in 0.06M phosphate buffer, 3%
sucrose (pH 7.4) with 0.15mM CaCl2 and then placed into 0.06M phosphate buffer, 15%
sucrose (pH 7.4) with 0.15mM CaCl2 for one hour at 4C. Eyes were then transferred to
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0.06M phosphate buffer, 30% sucrose (pH 7.4) with 0.15mM CaCl2 at 4C overnight.
Eyes were removed and were mixed in a 1:1 solution of 30% sucrose and OCT and then
transferred to a mixture completely comprised of OCT. Eyes were embedded in OCT
and then frozen using dry ice. Eyes were sectioned at 10m in thickness and placed onto
gelatin-coated slides.
Immunohistological analysisSections were removed from the freezer and air-dried for 2 hours. Slides were
then washed in PBS (pH 7.4), 5 minutes 3X and blocked in 5% normal goat serum (NGS)
in PBS with 0.3% Triton X-100 for 20 minutes at room temperature. Sections were then
incubated overnight with primary antibody diluted in blocking solution at 4C for 12-18
hours. Sections were then brought to room temperature and washed in PBS 15 minutes
4X. Secondary antibody diluted in blocking solution including the Hoechst nuclear dye
was applied, and slides were placed in 37C for 30 minutes. Sections were then washed
in PBS for 10 minutes 3X. Slides were mounted with Vectashield mounting medium and
stored in the freezer. Slides were analyzed using confocal microscopy and images were
captured digitally by Pamela Kainz. The following list includes the antibodies used, the
working dilution, and the cell types which possess the respective antigens: GFAP, 1:200,
Mller glial cells (primarily the cell endfeet); GS, 1:500, Mller cells. Secondary
antibodies used were AlexaFluor-488 or -555 conjugates.
Histology
Adult eyes were obtained using the method described above; however, the
fixative for this analysis contained 2.5% glutaraldehyde, 1% PFA in 0.06M PBS (pH
7.4), 3% sucrose, 0.15mM CaCl2. Isolated eyes were immediately transferred into fresh
cold fixative for 30 minutes. After this period, the eyes were placed in fresh fixative for
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2 hours. Eyes were then rinsed for 15 minutes 2X in 0.06M PBS (pH 7.4), 3% sucrose,
0.15mM CaCl2 and were then dehydrated in a graded series of ethanol in 0.06M PBS (pH
7.4), 3% sucrose, 0.15mM CaCl2 and infiltrated with propylene oxide and resin.
Transverse sections of 1m thick were collected and heat-mounted onto a gelatin-coated
glass slide and stained with 1% Methylene Blue, 1% Azure in 1% borax. Slides were
cover-slipped with DPX.
Larvae preparation for histological retinal analysis
Five-day old larvae were anesthetized in ice-cold fish water and fixed with 2.5%
glutaraldehyde, 1% PFA in 0.06M phosphate buffer (PBS) (pH 7.4), 3% sucrose,
0.15mM CaCl2 for 1.5 hours at 4C. Larvae were then rinsed in 0.06M PBS (pH 7.4), 3%
sucrose, 0.15mM CaCl2 2X five minutes. Larvae were dehydrated in a graded series of
ethanol in 0.06M PBS (pH 7.4), 3% sucrose, 0.15mM CaCl2 and infiltrated with
propylene oxide and resin. Transverse sections of 1m thick were collected and heat-
mounted onto a gelatin-coated glass slide and stained with 1% Methylene Blue, 1%
Azure in 1% borax. Slides were cover-slipped with DPX.
Visual behavioral analysis
The optokinetic reflex assay (OKR) was used to test the visual sensitivity of
larvae at 5 dpf. For testing, 4-5 subjects were transferred into small petri dishes
containing 5% methyl cellulose and placed within a drum lined with vertical black and
white stripes, 1cm in width. The drum was illuminated with a tungsten light source, 9.74
* 10-2
W/cm2
and a 2 minute trial was conducted, during which the direction of rotation
of the drum was switched 3-4 times. The criterion for a positive response was that each
larva either demonstrated a full smooth pursuit-saccade cycle or eye tracking movements
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in both the clockwise and counterclockwise directions when the drum was rotated
accordingly.
RESULTS
Mller glial cell expression of GFAP and GS is altered by -aminoadipic acid
To analyze the effects of-AAA on the adult zebrafish Mller cells, I exposed
several fish to different concentrations of the gliotoxin: 1mM, 10mM, and 25mM, 50mM
for time periods of 24 and 48 hours. A concentration of 50mM compromised severely
the overall health of the zebrafish and resulted in violent spasms. These fish were thus
sacrificed due to the fact that they appeared distressed and unhealthy. Fish exposed to
concentrations less than or equal to 25mM showed no behavioral abnormalities when
treated. These adults were fixed for retinal immunological and histological analysis.
Retinal sections were obtained, labeled with GS and GFAP, and imaged using
confocal microscopy and digital photography. Fish treated with the lowest concentration
(1mM) had retinas that appeared highly similar to wild type. Adults treated with the
highest, non-lethal concentrations (10mM and 25mM) also had retinas that appeared to
be well intact. To examine specifically Mller cells, antibodies to two known cell
specific proteins, GS and GFAP, were utilized. Exposure to 10mM -AAA for 24 hours
appeared to affect modestly the expression of GS and GFAP.
The retinal images shown in figure 2 were obtained from a specified region in the
dorsal part of the retina from treated and untreated animals. The expression of GS in
untreated retinas was evenly distributed throughout the Mller cell bodies and therefore,
the retina (Fig. 2a), while the expression of GS in treated retinas had a spoke-like pattern
(reminiscent of the Mller cell bodies) suggesting that the either the expression of this
protein increased in response to the gliotoxin or the size of the Mller cell processes
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increased (Fig. 2b). In addition, there appeared to be less GS labeling in the inner
plexiform synaptic layer in the treated retina compared to controls.
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Fig. 2. Zebrafish treated with 10mM -aminoadipic acid for 24 hours exhibited differences in GS (red) and GFAP(green) expression in comparison to controls. The photoreceptor layer (PRL) and inner-nuclear layer (INL) are labeled.a: GS expression in untreated retinas was evenly distributed in each layer of the retina. b: GS expression in treatedretinas appeared denser or spoke-like. c: GFAP expression in untreated retinas was confined to the Mller cellendfeet. d: GFAP expression in treated retinas was somewhat elevated in Mller cell bodies and in radial processes
reaching the outer-plexiform layer.
c
ba
d
INL
PRL
Endfeet
wt control
wt control
wt 10mM
wt 10mM
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More substantial differences were found in the expression of GFAP. In the
controls, immunoreactivity was mostly confined to the Mller cell endfeet (Fig. 2c).
However, in the treated retinas, the GFAP immunoreactivity was present throughout the
Mller cell bodies in radial processes reaching the outer plexiform layer (Fig. 2d)
suggesting that the expression of GFAP increased in response to exposure to the
gliotoxin, consistent with what would be predicted.
The pattern of Hoechst nuclear dye labeling shown in blue in figure 2c and 2d
illustrates how well-preserved the 10mM and 25mM -AAA treated retinas were
compared to untreated controls. No gaps were seen in the nuclear layers indicating that
-AAA did not result in massive cell death, and three distinct nuclear layers were
observed implying that retinal organization was not disrupted. In case the mild effect on
Mller cells disrupted their ability to support photoreceptors, I examined closely the
integrity of the photoreceptors cells in the treated animals. No evidence of photoreceptor
cell disruption was observed.
Increased dosage and a longer incubation period yielded similar results
The 24 hour exposure of 10mM and 25mM Mller appeared to have no major
detrimental effect on retinal neurons but did affect mildly Mller glia. Since the goal was
to determine whether -AAA could compromise significantly the Mller glia while
having no effect on retinal neurons, I decided to push the system. Since higher
concentrations were lethal, I chose to increase the length of exposure. For this, I exposed
adult zebrafish to a concentration of 25mM over a period of 48 hours and found that the
severity of the effect had not increased. Again, the expression of GS and GFAP were
mildly elevated (data not shown). Greatly increasing the exposure time may have
strengthened the gliotoxin affect; however, we did not feel this was a very practical
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approach given the large amount of drug we would need to utilize in order to be able to
change the 400mL solution of-AAA daily. Instead I set out to determine the effect -
AAA had on larval zebrafish.
When combined with constant light, -aminoadipic acid caused a similar phenotypeKnowing that constant and intense light exposure exacerbated the Mller cell
phenotype in the larval genetic model of Mller cell disruption, the lze mutant, I tested
the impact of combining pharmacological stress with light toxicity in the adult. Although
teleost retinas have shown more resistance to light damage than rodents (where the retina
is largely rod dominated), light toxicity has been studied in albino adult zebrafish where
it has caused rod and cone cell apoptosis (Vihtelic and Hyde, 2000). We chose to avoid
the use of albino zebrafish due to their low viability as larvae and extreme susceptibility
to light toxicity. Instead, I tested -aminoadipic acid treated and untreated adult wild
type zebrafish in a light regiment of 15,000 lux, nearly twice the intensity necessary to
observe photoreceptor cell death in albinos.
My initial result suggested that the combination of the toxin (25mM -AAA) and
constant light caused photoreceptor cell death in the adult zebrafish (Fig. 3). This was
apparent from observing a Hoechst nuclear dye that indicated that the dorsal portion of
the outer-nuclear layer was only one nucleus thick in -AAA light treated fish but 2-3
nuclei thick in controls (unexposed to light or the drug). When repeated several times,
the experiment provided new data to suggest that my light exposure regiment alone could
sometimes cause photoreceptor disruption and death (Fig. 4).
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Fig. 3. Adult zebrafish treated with 25mM -aminoadipic acid for three days under constant lighting conditions had
photoreceptor cell degeneration. a: The outer nuclear layer (ONL) in untreated retinas appears healthy and is
approximately three nuclei thick when viewed under a Hoechst stain. b: The ONL in the retina exposed to constantlight appears overall healthy to the control, with the layer spanned by a thickness of 2-3 nuclei. c: The ONL in theretina exposed to constant light and 25mM -aminoadipic acid is approximately one nucleus thick indicating that many
photoreceptors were lost. Pyknotic nuclei are indicated by arrows.
control
a
c
b
light
ONL
ONL
ONL
light/AAA light/AAA
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ba
c
OS
ONL
INL
GCL
Fig. 4. Adult zebrafish retinas exposed to constant
light exhibit a similar phenotype to those exposed to
constant light and 25mM -aminoadipic acid for
three days. a: The untreated retina exhibits healthy
outer segments (OS). b: The retina exposed toconstant lighting expresses unhealthy and missing
outer segments (arrow) and missing photoreceptornuclei. c: The retina exposed to constant lightingand treated with 25mM -aminoadipic acid was
similar to the retina treated with light alone, having
photoreceptor cell loss and outer segment
disru tion.
control light
light/AAAp
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Larval health was compromised at concentrations similar to the adult
Wild type larvae were treated with various concentrations of the toxin by adding
it to their water in petri dishes from 3 dpf to 5 dpf. Survival data is located in Table 1. I
found t
s
hat 81% of larvae survived a two day exposure at concentrations of 10mM and
61% survived a two day exposure at a concentration of 25mM. Survival percentage was
0% at 50mM, although 1/15 treated fish survived a concentration of 100mM (7%). Thi
non-lethal dose pattern was thus similar to adults.
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-Aminoadipic
Acid
Concentration
(48hr Exposure)
Wild Type Larvae
Treated
Wild Type Larvae
Survived
Survival
Percentage
0mM (control) 45 45 100%
10mM2 36 22 61%
15 0 0%
5mM
50mM
15 14 87%
100mM 15 1 7%Table 1. Wild type larvae have similar dosage dependent survival as adult z re able toexposure of 48 hours at concentrations up -aminoadipic acid before displayed scant survival. ly,t f adults was severely comprom t concentrations of 50mM or higher.
ebrafish. Larvae we tolerate anto 25mM they Similar
he health o
ised a
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General characteristics of 5 dpf-aminoadipic acid treated larvae
All of the treated larvae at 25mM appeared similar to untreated animals with
some exc ent and
lacked an inflated swim bladder. Furthermore, they demonstrated little spontaneous
activity and had only a moderate response to touch. The yolk of treated larvae was also
observed to be partitioned. Heart rate was found to be the same between treated and
untreated wild type larvae. The jaw twitching, lethargy, and under-inflated swim bladder
were all characteristics in common with the lze Mller glia mutant.
Wild type larvae treated with -aminoadipic acid demonstrate an OKR similar to controls
utilized the
o
demonstrated an almost identical response to the assay as untreated wild type controls
(when the light level in the barrel was not attenuated). Both untreated and treated larvae
demonstrated a strong saccade and steady tracking of the black and white stripes.
Alpha-aminoadipic acid causes disruptions in the ganglion cell layer, inner nuclear
While the visual behavior of treated and untreated wild type larvae was similar,
histologic xposed
to 10mM -AAA. Pyknotic nuclei, that appear darkened with a halo of empty space
surrounding them, were identified within the ganglion cell layer (GCL), indicating that
some of these neurons were degenerating (Fig. 5b). In addition, the toxin compromised
the marginal zone as indicated by gaps seen in this region where proliferative stem cells
are present in controls. At concentrations of 10mM, the toxin also appeared to have an
effect on the horizontal cell layer, causing large gaps, indicating the presence of fewer
horizontal cells compared to untreated larvae (Fig. 5b).
eptions. Treated larvae displayed a constant jaw twitching movem
To test the vision of wild type larvae treated with the toxin, I
ptokinetic reflex assay. I found that larvae treated at a concentration of 25mM
layer, horizontal cell layer, and marginal zone in zebrafish larvae
al findings showed that some retinal neurons were disrupted in larvae e
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Increasing the dosage of the drug proved to increase inner nuclear lay
disruption. At concentrations of 25mM, the toxin cause
er
d cell loss within GCL but also
caused death in INL (Fig. 5c). Large circular gaps were present in these treated retinas,
reminiscent of retinal locations where cell death had just occurred. Gaps in the brain
were observed in animals treated with 25mM -aminoadipic-acid (Fig. 5d).
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Fig. 5. Wild type zebrafish larvae retinas treated with -aminoadipic acid at concentrations of 10mM and 25mM an
for an incubation period of 48 hours expressed disruptions in the ganglion cell layer, inner nuclear layer, horlayer, and marginal zone. a: Control retinas showed no signs of cell death. b: Wild type retinas treated withconcentrations as low as 10mM expressed pyknotic cells in the ganglion cell layer (orange arrow), missing
cells (red arrow), and deficiencies in the marginal zone (green arrow). c: Increasing the dosage to 25mM
d
izontal cell
horizontal
resulted inmore inner nuclear layer deficiencies and large gaps. d: Concentrations of 25mM also caused larges gaps of missing
cells in the brain.
a
wt
control
b
wt
10mM
wt25mM wt25mM
dc
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Alpha-aminoadipic acid causes cell migration out of the retina through the optic
nerve in some wild type retinas
In two of the approximately 20 wild type treated retinas that were sectioned
(1 t0%), I observed cell migration out of the retina through the optic nerve. I could no
ascertain definitively the direction of the migration, although it appears as if cells were
funneling out of the retina towards the brain (Fig. 6a). Cells were elongated, which is
indicative of migrating cells, and some seemed to be differentiated. A cell associated
with an outer segment (a presumed photoreceptor) can be seen within the migratory
stream of cells (Fig. 6b). This effect was seen in wild type treated larvae at a
concentration of 10mM and at a concentration of 100mM but never in wild type untreated
larvae (data not shown).
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Fig. 6. In 10% of wild type treated retinas, -aminoadipic acid caused retinal cell migration out of the retina throughthe optic nerve. a: Differentiated and elongated cells appeared as though they were migrating out of the retina towards
the brain. b: A close up of the optic nerve region. The circle surrounds a cell with an outer segment, indicative of aphotoreceptor cell.
a
wt10mM wt10mM
b
wt10mM
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Alpha-aminoadipic acid does not seem to worsen severely the lze phenotypeSince the zebrafish is a genetic model organism, mutants, such as lazy eyes, could
be used to investigate the combined effects of genetic and pharmacological manipulation
of glia
e
on the neural retina. Knowing that lze mutants have compromised Mller glial
cells, I was curious whether-AAA would increase the severity of the lze Mller cell
phenotype. Thus, the same xperiments were carried out on lze larvae. Larvae from the
lze clutch that were treated with 10mM -AAA exhibited subtle histological
abnormalities within the spectrum of what was observed in treated wild type larvae and in
lze untreatedcontrols (Fig. 7).
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Fig. 7. Lze larvae treated with -aminoadipic acid exhibit a phenotype similar to lze untreated controls. a: Lze larvaetreated with 10mM -aminoadipic acid appear to have some inner nuclear layer deficiencies (highlighted by the arrow)
but do not appear severely different from lze controls. b: A lze control is pictured.
a
lze10mM
b
lzecontrol
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DISCUSSION
The goal of the work outlined in this chapter was to explore the gliotoxic effect of
-AAA on the retina using the zebr el. Previous studies using -AAA
have su
ed tepid effects, considerably weaker than those
observe
l cells out the optic nerve in a
afish animal mod
ggested that retinal glial cells were specifically affected; however, none have been
on the zebrafish nor have any been conducted without the use of invasive methods of
drug delivery such as intraocular injection. By delivering the drug via the fish water, the
concentration and thus dose of the drug at any one time is constant, unlike the
unavoidable fluctuation of drug dose with intraocular injection or subcutaneous injection
done in all previous in vivo studies. .
The investigation of an -AAA-mediated pharmacological model of Mller cell
disruption in the adult zebrafish yield
d in other animal models treated with the toxin. While other studies have
observed Mller cell death, swelling, or hypertrophy, as well as photoreceptor death, I
did not. My sole finding was a increase in the expression of GFAP. Although the
increase was subtle, upregulation of GFAP is a classic indication of Mller cell stress
indicating that the drug was having the desired affect. Furthermore, labeling with the GS
antibody revealed that Mller processes appeared thicker in response to treatment
suggesting that some degree of hypertrophy may have occurred. Thus, I observed signs
of Mller cell stress although these indications were more subtle than predicted.
Unfortunately the effects could not be increased in severity by increasing concentration
or length of exposure, before lethality became a problem.
In the wild type larval retina, I observed evidence of modest neuronal
degeneration. In addition, I noticed cell migration of retina
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few of
s the effects were very subtle in the adult retina and
detrime
the retinas. Both of these observations involved retinal neurons and indicated a
lack of glial-specificity. It is known that when -AAA is used at too high of a
concentration, the affects can be neurotoxic (Sugawara et al., 1990) perhaps indicating
that my dosage was too high. This is possible but unfortunately neither neurons nor glia
were affected by lower doses.
In summary, the effect of the gliotoxin varied substantially from fish to fish and
was highly dependent on age, a
ntal to retinal neurons in the larval zebrafish. Although more variables in
treatment strategy could be explored, the neurotoxic effects observed in the larvae
discouraged me from further pursuing this direction for the present time. As a result, I
focused on a different model of Mller cell stress mediated by a genetic mutant.
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Chapter 2: The Genetic Mode
INTRODUCTION
The impetus for mov ings of Rattner and Nathans
(2006) in their study on the gen eceptor stress induced either by
detachm
entation, and ocular homeostasis (Prasanna et al.,
2003).
ess.
In add
ing in this direction were the find
es related to photor
ent, genetic photoreceptor mutations, or light toxicity. Using microarray
technology, RNA blots, and in situ hybridization, they quantified the genomic responses
to both light damage and inherited photoreceptor degeneration and found that these
responses involve a relatively small number of overlapping genes (Rattner and Nathans,
2005). In their research, they discovered that the endothelin pathway is highly linked to
photoreceptor and Mller cell stress.
Endothelins are vasoactive peptides with various functions throughout vertebrates
including cardiovascular systems, pigm
There are three isoforms of the peptide: endothelin 1, 2, and 3. Endothelin
receptors come in two subtypes, endothelin receptors A and B, both G-protein coupled
receptors (Sakurai et al., 1992). In the retina, endothelin receptor A (ET-A) is mainly
localized to the choroid and blood vessels, whereas endothelin receptor B (ET-B) has
been found mainly in the neural and glial components of the retina (Maccumber and
DAnna, 1994) although the precise roles endothelins play in the retina are unknown.
Using the mouse model, Rattner and Nathans found that endothelin 2 is expressed
in photoreceptor cells and highly induced in all of their models of photoreceptor str
ition, they found that ET-B localized to Mller cells and its expression was
upregulated >10 fold following phototoxic conditions. These data led the authors to the
hypothesis that the endothelin pathway plays a critical role in the Mller cell response to
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stressed or dying photoreceptor cells and may be involved in the neuroprotective support
function Mller glia provide for photoreceptors.
Other studies have shown that the endothelin pathway is susceptible to
pharmacological manipulation. When administered to albino mice under phototoxic
conditi
spired my investigation of the ET-B knockout
zebrafi
ons, Tezosentan, a mixed ET-A and ET-B antagonist, lowered the amount of
GFAP expression and also resulted in a lower amount of apoptotic cells throughout the
retina, as judged by a CC3 cell death assay. These findings imply that inhibition of
endothelinergic receptors could play a role in the preservation of vision by sparing
photoreceptors (Torbidoni et al., 2005). The investigators hypothesized that the
endothelin pathway triggers the Mller cells to upregulate GFAP expression resulting in a
scarring effect and that the prevention of the Mller cell processes could promote
neuronal survival and preserve vision.
Strong associations between the endothelin pathway, Mller cells, and
photoreceptor support mechanisms in
sh called rose. Using a genetic mutant allowed me to circumvent some of the
drawbacks with a pharmacological model, specifically the variability and fluctuation in
drug concentration caused by metabolism. Rose was initially discovered through its
abnormal body pigmentation and the initial study concluded thatthe only defect caused
by the absence of the ET-B was the lack of the production of a subset of the adult
melanocytes and iridiphores. This phenotype resulted in adults appearing reddish
compared to wild type (Fig. 8) (Parichy et al, 2000). Later studies provided data to
support that the ET-B gene is actually expressed in the zebrafish larval retina (Lister et
al., 2006).
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type and rose mutant adult zebrafish (Source: Parichy et al., 2000)
. b: Rose mutants fail to develop the normal amount of melanocypattern metamorphosis, accounting for their reddish appearance.
Fig. 8. Wild . a: Wild type adults demonstratenormal coloring tes and iridophores during pigment
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In the second chapter of this study, I characterized the homozygous ET-B mutant
se zebrafish larval retina. Research on the links between phototoxicity and
photore
Wild type and rose homozygous recessive zebrafish were maintained as described
in Chapter 1.
Adult larvae were maintained in a standard 14/10-hour light-dark cycle until 2 dpf
when they were transferred to constant dark conditions because pretreatment with
constant darkness intensifies the effect of the light treatment to follow. Dark adaptation
ro
ceptor stress in addition to lzes increased Mller specific susceptibility to light
provided the impetus for exposing my genetic model to constant light. Rattner and
Nathans findings, that the endothelin pathway was involved in the response to
phototoxic condition, gave me further reasons to test how a retina missing ET-B would
react to constant lighting. I employed histological, behavioral, and quantitative
measurements to characterize the degree to which the health or function of the retina was
compromised. The OKR was used to measure the visual threshold of light-treated rose
mutants and control retinas, and these results were compared to wild type larvae under
the same two conditions: constant light (LL) and a normal light dark cycle (LD). Retinal
histology of rose was performed and cell counts on the inner and outer nuclear layers
were used to assess the presence or absence of cell death in the regions of the retina
containing Mller cells and photoreceptor cells. These experiments continue with the
theme of this thesis: exploring potential models where Mller cells are compromised and
observing the effects of this stress on photoreceptors and on vision in the zebrafish.
MATERIAL AND METHODS
Zebrafish maintenance
Constant light rearing
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fr ay 0 until day 2 was not necessary since larvae lack developed photoreceptors at
this point and opsin does not appear until 48hrs post fertilization (Schmitt et al., 1999).
At 4 dpf, larvae treated with constant light were transferred to a box lined with several
fluorescent bulbs and a fan used to minimize heat generated by the light. The light level
was approximately 15,000 lux, about 50 times brighter than average room light. Controls
were kept in standard light dark conditions from 2-6 dpf. Larvae were removed at 6 dpf
for visual testing and fixation.
Visual Threshold Assay
om d
All OKR assays were run on 6 dpf larvae between the hours of 1 PM and 5 PM in a
completely darkened room. I used a dim, red head-lamp for visibility when needed. For
testing, 4-5 subjects were transferred into small petri dishes containing 5% methyl
cellulos
Six-day old larvae were fixed using the same protocol as Chapter 1.
Cell Counts
ted
retinas in the inner and outer nuclear l nuclear layer counts did not register
e and placed within a drum lined with vertical black and white stripes, 1cm in
width. The drum was illuminated with a tungsten light source, 9.74 * 10-2 2
W/cm ,
attenuated by 6.5 log units, and the drum was rotated at 10 rpm. A 2 minute trial was
conducted, during which the direction of rotation of the drum was switched 3-4 times.
The lowest light level that evoked an OKR response for each larva was determined. The
criterion for a positive response was that each larva either demonstrated a full smooth
pursuit-saccade cycle or eye tracking movements in both the clockwise and
counterclockwise directions when the drum was rotated accordingly. Fish that failed to
demonstrate a positive response were retested using 0.5 log unit brighter illumination.
Histology
Cell counts were completed in rose and wild type light treated and untrea
ayers. Inner
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horizon one contains
proliferative stem cells, while the i layer contains Mller, bipolar, and
amacrine nuclei.
tal cells or nuclei in the marginal zone (Fig. 9). The marginal z
nner nuclear
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yer cell counts were performed is enclosed in red. Innerto include nuclei in the marginal zone (top arrow) or
Fig. 9. The region of the retina in which inner nuclear lanuclear layer nuclei were counted with careful attention not
horizontal cell nuclei (bottom arrow) in the count.
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RESULTS
Rose larvae have normal retinal morphology and visual function
Morphologically, rose and wild type larvae retinas were nearly indistinguishable
when the larvae were raised in a normal light dark cycle (Fig. 10a, 10c). Both had
healthy photoreceptors, a continuous span of nuclei in the outer and inner nuclear layers,
and he
althy, dense, and organized rod outer segments. Furthermore, without dark
adaptation and light attenuation, rose larvae responded equally robustly to wild type in
response to the OKR.
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constant light.ge
pe larvae treatede larvae treated
ment
Fig. 10. Wild type and rose larvae are strikingly similar when raised in a normal light dark cycle or witha: Wild type larvae raised in normal light dark cycle. Encircled is the rod dense ventral portion of the retina. Larrod outer segments span the region containing melanin from the pigmented epithelial cells. b: Wild tywith light. c: Rose mutant larvae kept in normal lighting conditions appear nearly identical to wild typ
in the same conditions. d: Rosemutant larvae treated in constant light show significant loss of rod outer segmaterial in the ventral retina.
wt LD wt LL
roseLD roseLL
a
c d
b
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When raised in constant light,rose showed higher susceptibility to rod outer
segment damage
Histological analysis of retinas from rose larvae exposed to constant light
vealed that there were limited but visible differences between rose and wild type retinas
(Fig ons
that ma
s of rod outer segment health. Some appeared
slightly
re
. 10b, 10d). Both retinas appeared grossly normal and neither displayed indicati
ssive cell death had occurred, in the form of pyknotic nuclei or gaps in the nuclear
layers. There were also no obvious signs of disruption within Mller cells. Their cell
bodies did not appear hypertrophied.
There was, however, one clear difference between retinas from constant light
reared wild type and rose larvae: the integrity of their rod outer segments. Rose light
treated retinas showed several degree
swollen in comparison to light dark treated rose larvae (Fig. 11). Most, however,
were disorganized, and many retinas were missing rod outer segments. Furthermore,
vacuoles within the RPE were very common. In contrast, the rod outer segments of wild
type light treated retinas almost always appeared equally healthy to their light-dark
counterparts. In some wild type retinas, there were slightly swollen or disorganized rod
outer segments; however, in only one of sixteen retinas were there actually fewer rod
outer segments.
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Fig. 11. Rose mutant larvae treated with constant light showed varyouter segments appear healthy and organized yet a few small vacuoles
segments appear substantially disorganized, shortened, and dysmorc: Significant loss of rod outer segments from the ventral retina has ta
a
roseLL
b
croseLL
roseLL
ing degrees of rod outer segment health. a: Rodappear in the RPE (red arrow). b: Rod outer
phic (orange arrow), and the RPE contains vacuoles.ken place.
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When treated with constant light,rose larvae had a 10% reduction in inner nuclear layer
nuclei, while the amount of inner nuclear layer nuclei in wild type remained constant
The lack of gaps in the nuclear layers and the absence of pyknotic nuclei suggest
t cell death in the rose retina did not occur, at least not on day 6 when the larvae were
s
of nucl
tha
acrificed. To ascertain whether any cell death had occurred prior to day 6, the number
ei were counted in the nuclear layer that contains the photoreceptor nuclei and the
nuclear layer that contains Mller cells. Average numbers were compared among light-
dark (LD) and light-light (LL) treated rose and wild type animals. Neitherrose nor wild
type showed a decrease in the number of outer nuclear layer (ONL) nuclei upon the
introduction of constant light; however, wild type had on average had more ONL nuclei
than rose in both treatment groups. For instance, rose light treated larvae had an average
of 156 ONL nuclei, while wild type had an average of 183, 20% higher with a p-value of
0.00022 (Fig. 12, Table 2).
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Fig. 12. Neitherrose nor wild type larvae lost photoreceptor nuclei upon treatment with constant light. Although theaverage number of nuclei in the ONL in rose LD and LL was different than wild type, no difference was observed
between rose LD and LL. Error bars represent 95% confidence intervals, and starred bars connect treatment groups forwhich there was a statistically significant difference in outer nuclear layer.
Rose and Wild Type Outer Nuclear Layer
wt LD wt LLroseLD rose LL
100
110
120
130
140
150
160
170
180
190
200
AverageNumberofNucleiinON
**
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rose LD rose LL wt LD wt LL
INL ONL INL ONL INL ONL INL ONL
Average
Number of Nuclei 385 161 349 156 339 179 358 183
Standard
Deviation 50 24 36 12 34 19 31 18
sNumberObservation 20 8 38 17 14 17 13 13
idence95% ConfInterval
[363,407]
[144,178]
[338,361]
[151,162]
[321,357]
[170,188]
[342,375]
[174,193]
Tabl e inner and ou nuclear r nucle rose and pe larvae across the two treatment groups.e 2. Averag ter laye i for wild ty
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Untreated rose larvae had an average of 385 nuclei in their INL in contrast to light
eated rose which had an average of 349 nuclei, roughly a 10% decrease. This
ifference was found to be significant to a p-value of 0.0092 (Fig. 13, Table 2). No such
effect w
tr
d
as observed in wild type light treated larvae. Another finding was that untreated
rose larvae had nearly 14% more INL nuclei than their untreated wild type counterparts,
which had an average of 339 nuclei. This difference was significant to a p-value of
0.0037 (Fig. 13, Table 2).
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Fig. 13. When treated with constant light, rose larvae lose 10% of their inner nuclear layer nuclei. Error bars represent95% confidence intervals, and starred bars connect treatment groups for which there was a statistically significantdifference in inner nuclear layer nuclei. Rose untreated larvae had an average of 385 inner nuclear layer nuclei, whilerose light treated larvae had an average of 349 inner nuclear layer nuclei (p-value 0.0092). There was also a
statistically significant difference between rose untreated larvae and wild type untreated larvae which had an average of339 nuclei (p-value 0.0037).
Rose and Wild Type Inner Nuclear Layer
wt LD wt LLrose LD rose LL250
270
290
310
330
350
370
390
410
AverageNumberofNucleiinth
eIN
****
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Untreatedrose larvae exhibit a lower visual threshold thanrose larvae treated with
constant light; wild type shows no loss in visual function after light treatment
While I had observed that untreated rose and wild type exhibited equally robust
ponses to the OKR without dark adaptation, I realized that this was only a qualitative
visual
rvae raised in a normal
light da
res
observation. To obtain a quantitative assessment of visual behavior, I chose to measure
thresholds. Thresholds were found by determining the lowest light level that
evoked an OKR response for each larva. Larvae that failed to demonstrate a positive
response were retested using 0.5 log unit brighter illumination.
In light-dark conditions, rose and wild type exhibited an average threshold of -6.0
log units of light attenuation similar to wild type (Fig. 14, Table 3). When reared in light-
light, rose larvae had a significantly higher threshold than rose la
rk cycle and than wild type larvae treated in constant light. Rose light treated
larvae had an average threshold of -4.5, while untreated rose larvae had an average
threshold of -6.0 (Fig. 14, Table 3). This difference was highly significant to a p-value of
2.8 * 10-7
. In addition, this drop in visual sensitivity was not seen in wild type suggesting
that the light-light treatment used had no measurable effect on fish having an intact ET-B
gene. Light treated wild type larvae had an average threshold of -5.8. The difference
between rose and wild type light treated larvae was significant to a p-value of 2.7 * 10-6
.
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Fig. 14. When treated with constant light, the visual threshold ofrose larvae increases. In contrast, constant light doesnot affect the visual sensitivity of wild type larvae. Error bars represent 95% confidence intervals, and starred barsconnect treatment groups for which there was a statistically significant difference in visual threshold. Rose light treated
larvae had an average threshold of -4.5, while untreated rose larvae had an average threshold of -6.0 (p-value of 2.8 *10
-7). There was also a statistically significant difference between rose light treated larvae and wild type light treated
larvae, which had an average threshold of -5.8 (p-value of 2.7 * 10-6).
Rose and Wild Type Visual Threshold
wt LD wt LLrose LD rose LL3.0
3.5
4.0
4.5
5.0
5.5
6.0
6.5
AverageThreshold(UnitsofNegativeLog
Attenuation
)** **
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rose LD rose LL wt LD wt LL
Average Threshold -6 -4.5 -6 -5.8
Standard Deviation 0.5 1.5 0.5 0.5
Number Observations
rval [-5.8 [-4.1, -5.0] [-5.8, -6.2] [-5.7, -6.0]-5 or Lower
97% 45% 100% 94%
Number Thresholds HigherThan -5 1 23 0 2
55%
29 42 30 33
95% Confidence Inte , -6.2] Number Thresholds 28 19 30 31
% Thresholds -5 or Lower
% Thresholds Higher Than -5 3% 0% 6%Table 3. Average visual threshold forrose and wild type larvae across the two treatment groups.
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Rose light treated larvae in general varied substantially in their thresholds. Some
ad thresholds equivalent to wild type, while others had significant drops in their visual
nsitivity. To illustrate this phenomenon, I calculated the percent of larvae in each
group t
h
se
hat had a threshold of -5 or lower. I used -5 as cutoff because this is the highest
threshold any light-dark wild type larva ever demonstrated. While rose untreated larvae,
wild type untreated larvae, and wild type light treated larvae had thresholds of -5 or lower
in 97%, 100%, and 94% of the data points respectively, rose light treated larvae only had
a threshold of -5 or lower 45% of the time (Fig. 15, Table 3). The difference between
rose light treated and rose untreated larvae in this case was significant to a p-value of 1.4
* 10-7
, a highly robust result.
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Fre
Roseand Wild Type Visual Threshold Binomial Data
wt LD wt LLrose LD rose LL
0.0%
20.0%
40.0%
60.0%
80.0%
100.0%
tof
shol
rLowe
ds-5o
Thre
Percen
ig. 15. The percentage of larvae in each treatment group that had a threshold of -5 or lower is depicted. Error barspresent 95% confidence intervals. While 97% of untreated rose larvae had a threshold of -5 or lower, only 45% ofe light treated rose larvae had a threshold of -5 or lower (p-value 1.4* 10-7).th
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Inner nuclear layer count and visual threshold are not correlated inrose light treated larvae
Curious whether there was relationship between the loss of cells in the INL and
high visual thresholds, I tested rose light treated larvae in the OKR and separated them
into two groups, those with a threshold of -5 or lower and those with a threshold higher
than -5. I then proceeded to calculate the average number of INL nuclei in each group.
There did not appear to be a correlation between INL count and visual threshold as both
groups expressed a nearly identical average number of nuclei (Fig. 16, Table 4).
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Inner Nuclear Layer Visual Threshold Correlation
Rose LL Low
Threshold
Rose LL High
Threshold250
270
290
310
330
350
370
390
AverageNumberofNucleii
nINL
Fig. 16. When rose light treated larvae were separated into two groups, those with visual thresholds of -5 or lower
(Low Visual Threshold) and those with visual thresholds higher than -5 (High Visual Thresholds), there was nosignificant difference in the average number of inner nuclear layer nuclei across the two groups. Error bars represent95% confidence intervals.
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rose LL Low
Visual Threshold
rose LL High
Visual Threshold
Average Number of Nuclei in INL 356 358
Standard Deviation
Number Observations
[330, 382] [342, 374]
35
7
31
15
95% Confidence IntervalTable 4. Average number of nuclei in the inner nuclear layer across rose ae with visual thresholds of- old) or with visual thresholds higher than igh Visual Threshold).
light treated larv-5 (H5 or lower (Low Visual Thresh
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DISCUSSION
In my evaluation of rose, I discovered several interesting characteristics of the
utant. The first was its striking similarity to wild type. ET-B thus is apparently not
m the absence of ET-B did result in
onic hydrase II, to retinal sections from rose treated and untreated retinas
to asce
pment
(Bilotta
m
necessary for early retinal develop ent. However,
decreased photoreceptor resistance to light damage. Rose had compromised rod outer
segments and a higher visual threshold than wild type. The final observation about the
rose mutant was its INL vulnerability to constant light. While wild type showed no loss
of INL nuclei in response to light treatment, the average number of nuclei decreased by
10% in rose. Thus, the absence of ET-B does indeed compromise the retinas resilience.
At this point however, I have not yet proven that this phenotype is related specifically to
Mller cells.
The nuclei that reside in the inner nuclear layer belong to bipolar, horizontal,
amacrine, and Mller cells. As a final experiment, I applied a Mller cell-specific
antibody, carb
rtain whether Mller cells were likely the cell type that was missing or partially
missing. While this experiment was attempted twice, I was unable to obtain any labeling
of Mller cells in rose retinas using this antibody, for reasons I do not understand.
The most logical explanation for a higher visual threshold is fewer
photoreceptors. Most research has implicated cones as the predominant contributor to
visual sensitivity at 6 dpf since they greatly outnumber rods at this stage in develo
et al., 2001). However, if the visual sensitivity problems had been cone related, I
would have observed a difference in ONL nuclei, which I did not. The only differences I
observed were manifested in rods, specifically in the health of their outer segments. This
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lead us to believe that although there were no pyknotic rod nuclei in the ONL, the
disorganization and scarcity of the rod outer segments in rose light treated retinas could
imply that the rods were significantly compromised and that rods may play a significant
role in visual function at this stage in development. Therefore, we believe that higher
visual threshold was likely a result of compromised rod outer segment health.
When assessing the reasons behind the rose mutants vulnerability to light
toxicity, we could not ignore that fact that rose has a deficiency in cells which are
pigmen
neuroprotective program, perhaps
mediate
ted: melanocytes and iridiphores. Thus, perhaps rose is more sensitive to light
damage merely because it is missing melanin in the retinal pigmented epithelial cells,
much like the albino model. I did not observe evidence in support of this possibility as
the melanin density in the retinal pigment epithelium in rose retinas did not appear
different from that which was observed in wild type.
A second hypothesis which we think holds more promise and that is consistent
with the literature is that ET-B is involved in a
d by Mller cells as implied by the results from mouse models. To follow this
idea, I would first need to confirm that Mller cells express ET-B in the zebrafish retina.
Then, I would want to explore how and whether this expression level changes as a result
of intense light exposure. If the expression of ET-B were specific to Mller cells and
increased in response to light exposure, more experiments would be needed to explore the
timing of rod photoreceptor cell disruption and the loss of INL nuclei to gain a better
understanding of how endothelins and Mller cells are involved in neuroprotection within
the retina.
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FUTURE EXPERIMENTS
As m
entioned above, insitu hybridization experiments are needed to confirm the
xpression of ET-B in Mller cells. The findings of Rattner and Nathans on the
association between ET-B an research on the pig retina,
tment, prior to day 5 when the animals were sacrificed.
To do t
phenotype, I could combine this model with a morpholino gene knockdown approach,
e
d Mller cells, in addition to
which found ET- B to be expressed by the innermost retinal layers, ganglion cell somata,
and by Mller glial cells (Iandiev et al., 2005), have provided compelling circumstantial
evidence that ET-B would be expressed by zebrafish Mller cells. However, other
studies have demonstrated that ET-B is also expressed in other cells within the mouse
retina, including horizontal cells and the retinal pigment epithelium (Torbidoni et al.,
2005). Thus, I would need to investigate this possibility in the zebrafish. After obtaining
the pattern of ET-B expression in the wild type zebrafish retina, I would repeat the
analysis of ET-B expression on rose larvae that had been exposed to constant light to
determine whether Mller cells or any other ET-B positive cells had an appreciable
change in expression level. This would help to identify the cell type(s) involved in the
response to photoreceptor stress.
Next, I would like to determine the identity of the missing cells within the INL in
light-treated rose larvae. One possibility explaining the absence of these cells is that cell
death had occurred during the trea
his, I would use a TUNEL cell death assay on retinas from rose larvae exposed to
light for different periods of time and use cell-specific markers to determine the identity
of TUNEL positive cells.
Once I had more knowledge of the basis for the light-treated rose retinal
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targeting candidate genes thought to be involved in the endothelin pathway. Another
potentially interesting experiment would be to introduce the rose mutation to the lze
enotype.
mutant to explore the effects of combining models involving Mller cells and light-
dependent degeneration.
Finally, since many of the genes in the zebrafish have more than one copy, I
might learn that there is more than one gene for ET-B. In this case, I would repeat the
experiment and analysis using rose larvae treated with a known ET-B inhibitor, called
BQ788, and assess the ph
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GENERAL CONCLUSIONS
To examine how Mller cells may be involved in supporting photoreceptors,
liable models where Mller cells are compromised are needed. In this thesis, I
xamined two candidate models of Mller cell disruption in the zebrafish retina, one
pharmacological and one gen ced a gliotoxin to adult and
larval z
mal models. Thus, even if I determine that the rose phenotype is not
mediate
cells
has ins
re
e
etic. In my first model, I introdu
ebrafish through the water and observed modest signs of Mller cell stress in the
adults but neuronal deficits in the larval retina. Because my approach did not yield the
desired glial-specific effects I had hoped to achieve, I chose to focus my attention on the
rose mutant model.
Upon the introduction of retinal stress via constant light, photoreceptor cells and
cells within the INL were compromised in the rose retina. The appearance of the failing
rod photoreceptor outer segments is similar to early stages of photoreceptor degeneration
observed in other ani
d by Mller cell deficiencies, rose still serves as a model of photoreceptor
degeneration, where the same issues of neurotrophic support could be investigated.
Whetherrose will be a useful model to study how Mller cells are involved in the
resilience of photoreceptors has yet to be determined; however, my finding that rod
photoreceptors were more vulnerable to phototoxic stress coupled with the Rattner and
Nathans result that light exposure led to the intense upregulation of ET-B in Mller
pired me to explore more about this mutant.
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