Visualization of the Superior Ocular Sulcus during Danio rerio Embryogenesis

Kevin  H. Yoon; Sonya  A. Widen; Melissa  M. Wilson; Jennifer  C. Hocking; Andrew  J. Waskiewicz

doi:10.3791/59259

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W tym Artykule

Podsumowanie
Streszczenie
Wprowadzenie
Protokół
Wyniki
Dyskusje
Ujawnienia
Podziękowania
Materiały
Odniesienia
Przedruki i uprawnienia

Podsumowanie

Here, we present a standardized series of protocols to observe the superior ocular sulcus, a recently-identified, evolutionarily-conserved structure in the vertebrate eye. Using zebrafish larvae, we demonstrate techniques necessary to identify factors that contribute to the formation and closure of the superior ocular sulcus.

Streszczenie

Congenital ocular coloboma is a genetic disorder that is typically observed as a cleft in the inferior aspect of the eye resulting from incomplete choroid fissure closure. Recently, the identification of individuals with coloboma in the superior aspect of the iris, retina, and lens led to the discovery of a novel structure, referred to as the superior fissure or superior ocular sulcus (SOS), that is transiently present on the dorsal aspect of the optic cup during vertebrate eye development. Although this structure is conserved across mice, chick, fish, and newt, our current understanding of the SOS is limited. In order to elucidate factors that contribute to its formation and closure, it is imperative to be able to observe it and identify abnormalities, such as delay in the closure of the SOS. Here, we set out to create a standardized series of protocols that can be used to efficiently visualize the SOS by combining widely available microscopy techniques with common molecular biology techniques such as immunofluorescent staining and mRNA overexpression. While this set of protocols focuses on the ability to observe SOS closure delay, it is adaptable to the experimenter's needs and can be easily modified. Overall, we hope to create an approachable method through which our understanding of the SOS can be advanced to expand the current knowledge of vertebrate eye development.

Wprowadzenie

The formation of the vertebrate eye is a highly conserved process in which carefully orchestrated intercellular signaling pathways establish tissue types and specify regional identity¹. Perturbations to early eye morphogenesis result in profound defects to the architecture of the eye and are frequently blinding². One such disease results from the failure to close the choroid ocular fissure in the ventral side of the optic cup³. This disorder, known as ocular coloboma, is estimated to occur in 1 out of 4-5000 live births and cause 3-11% of pediatric blindness, commonly manifesting as a keyhole-like structure that protrudes inferiorly from the pupil in the center of the eye⁴^,⁵^,⁶. The function of the choroid fissure is to provide an entry point for early vasculature growing into the optic cup, after which the sides of the fissure will fuse to enclose the vessels⁷.

While ocular coloboma has been known since ancient times, we have recently identified a novel subset of coloboma patients with tissue loss affecting the superior/dorsal aspect of the eye. Recent work in our lab has led to the discovery of an ocular structure in the zebrafish dorsal eye, which we refer to as the superior ocular sulcus (SOS) or superior fissure⁸. It is important to note that the structure has characteristics of both a sulcus and a fissure. Similar to a sulcus, it is a continual tissue layer that spans from the nasal to the temporal retina. In addition, the closure of the structure is not mediated by a fusion of the two opposing basement membrane, and it appears to require a morphogenetic process by which the structure is populated by cells. However, similar to a fissure, it forms a structure that separates the nasal and temporal sides of the dorsal eye with the basement membrane. For consistency, we will refer to it as SOS in this text.

The SOS is evolutionarily conserved across vertebrates, being visible during eye morphogenesis in fish, chick, newt, and mouse⁸. In contrast to the choroid fissure, which is present from 20-60 hours post-fertilization (hpf) in zebrafish, the SOS is highly transient, being easily visible from 20-23 hpf and absent by 26 hpf⁸. Recent research in our lab has found that, similar to the choroid fissure, the SOS plays a role in vascular guidance during eye morphogenesis⁸. Although the factors that control the formation and closure of the SOS are not yet fully understood, our data did highlight roles for dorsal-ventral eye patterning genes⁸.

Zebrafish is an excellent model organism to study the SOS. As a model system, it provides a number of advantages in studying eye development: it is a vertebrate model; each generation exhibits high fecundity (~200 embryos); its genome has been fully sequenced, which facilitates genetic manipulation; and approximately 70% of human genes have at least one zebrafish orthologue, making it an ideal genetics-based model of human disease⁹^,¹⁰. Most importantly, its development takes place externally to the mother, and its larvae are transparent, which allows for the visualization of the developing eye with relative ease¹¹.

In this set of protocols, we describe the techniques through which the SOS can be visualized in zebrafish larvae. The variety of visualization techniques used in this report will allow clear observation of the SOS during normal eye development, as well as the ability to detect SOS closure defects. Our example protocols will feature investigations of Gdf6, a BMP localized to the dorsal eye and known regulator of SOS closure. Further, these techniques can be combined with experimental manipulations to identify genetic factors or pharmacological agents that affect proper SOS formation and closure. In addition, we have included a protocol through which the fluorescent imaging of all cell membranes is possible, allowing the experimenter to observe morphological changes to the cells surrounding the SOS. Our goal is to establish a set of standardized protocols that can be used throughout the scientific community to offer new insights into this novel structure of the developing eye.

Protokół

All methods described here have been approved by the University of Alberta Animal Care and Use Committee.

1. Protocol 1: Visualization of SOS using stereomicroscopy and differential interference contrast (DIC) imaging

Embryo collection
1. In a tank of dechlorinated water, prepare crosses of gdf6a^+/- zebrafish in the evening by pairing a male zebrafish with a female zebrafish. Be sure to separate the male from the female by using a divider to ensure that the embryos are born within a small range of time.
2. The following morning, pull the divider and allow the zebrafish to breed for no longer than 30 min. Collect the embryos in Petri dishes with E3 media, described in The Zebrafish Book¹², and place them in a 28.5 °C incubator.
3. Remove any unfertilized eggs or dead embryos, which will appear white and opaque.
Preparation and live-imaging of zebrafish embryos
1. At 20 hpf, replace the E3 media with E3 media containing 0.004% 1-phenyl 2-thiourea (PTU) to prevent pigment production.
  NOTE: Addition of PTU at a slightly later timepoint, such as 22-24 hpf, is unlikely to interfere with the experiment due to the early age of the embryos at the time of imaging. However, it is recommended to treat the embryos early to completely prevent pigmentation as there is a band of pigmentation that appears in the dorsal eye, which can interfere with the imaging of the SOS.
2. Ensure that all embryos are at the correct developmental stages at various points leading up to the time of observation. It is recommended that this is done at the stages at which somite number is clearly visible as outlined by Kimmel et al.¹³. Remove those that are developmentally immature.
3. Place the embryos under a dissecting microscope, and dechorionate the embryos by gently pulling apart the chorion using fine forceps. Visualize the SOS in the dorsal eye. The SOS may appear as an indentation at the dorsal margin of the eye, and a line should be visible across the dorsal eye. For normal SOS closure, observe the embryos at around 20-23 hpf. For examination of delayed SOS closure phenotypes, observe the embryos at 28 hpf or later.
4. Sort the embryos that show SOS closure delay from those that do not.
5. To photograph these embryos using a dissecting microscope, prepare a Petri dish containing 1% agarose in E3. Lightly prick the center of the agarose to create a shallow hole in which the yolk of the embryo can sit when the embryo is placed on the agarose. This will ensure that the embryo is not at an oblique angle when being photographed.
6. Anesthetize embryos with 0.003% tricaine in E3 and place laterally on the agarose.
7. To image the embryos using a compound or confocal microscope, transfer the embryo into 35 mm Petri dish containing a small bolus of non-gelled 1% low-melting point agarose in E3 (w/v). Quickly position the embryo laterally using a fine fishing line or an eyelash and wait for the agarose to cool. Once the agarose is firm, pour enough E3 into the dish to cover the agarose. For more details, see Distel and Köster¹⁴.
  NOTE: If using an inverted microscope, the embryo can be placed against the glass of a glass-coverslip-bottom dish and imaged with a standard 20X objective lens.
8. Use a water immersion 20x objective lens to visualize the SOS with a compound microscope. Following visualization, gently pull the agarose from the embryos and fix in 4% paraformaldehyde (PFA) or allow to continue their development.

2. Protocol 2: Whole-mount immunofluorescent staining of laminin

Whole-mount immunofluorescent staining of laminin: Day 1
1. Dechorionate embryos as described in Step 1.2.3, if not already done. Fix embryos in a microcentrifuge tube at the desired timepoint in freshly made 4% PFA for 2 h on a room temperature (22-25 °C) shaker. Wash in 1x PBST for 5 min, four times.
  NOTE: Following gastrulation, embryos may fix better after dechorionation.
2. Permeabilize embryos in 10 µg/mL proteinase K at room temperature for 5 min. Incubation time will depend on the developmental stage at which the embryos are fixed (see Thisse and Thisse¹⁵).
3. Wash in 1x PBST for 5 min, four times.
4. Block embryos in a solution of 5% goat serum and 2 mg/mL bovine serum albumin (BSA) in 1xPBST for 1-2 h on a room temperature shaker.
5. Prepare primary antibody solution by diluting rabbit anti-laminin antibody in block solution at a 1:200 dilution.
6. Incubate the embryos in anti-laminin primary antibody overnight on a 4 °C shaker.
Whole-mount immunofluorescent staining of laminin: Day 2
1. Wash in 1x PBST for 15 min, five times.
2. Prepare secondary antibody solution by diluting goat anti-rabbit Alexa Fluor 488 antibody in 1x PBST to a dilution of 1:1000.
  NOTE: It is possible to adapt this step to suit the resources available to the experimenter by using a different secondary antibody.
3. Incubate the embryos in secondary antibody overnight on a 4 °C shaker. Shield from light as much as possible from this step onwards.
4. Wash in 1x PBST for 15 min, four times. The embryos can be stored at 4 °C for up to a week, if necessary.
Dissection and mounting of embryonic eyes
1. If desired, place the embryos in a small Petri dish and deyolk the embryos in 1x PBST. Do this by gently disrupting the yolk with fine forceps and removing the yolk cells through mild scraping of the yolk sac.
2. Prepare the following concentrations of PBS-glycerol series solutions in microcentrifuge tubes: 30%, 50%, and 70% glycerol in PBS. Transfer embryos into 30% glycerol/PBS, making sure to place the embryos on top of the solution and transferring as little of the previous solution as possible. Wait for the embryos to sink to the bottom of the tube.
3. When embryos have sunk to the bottom, transfer them to 50% glycerol/PBS. Repeat and transfer to 70% glycerol/PBS.
4. Once the embryos have sunk in 70% glycerol/PBS, move them to a small plastic dish for dissections.
5. Sever the embryo posterior to the hindbrain, and use the posterior tissue for genotyping, if necessary.
6. Move the head to a glass slide, transferring as little glycerol as possible. Use forceps or other fine dissection tools to hold onto the posterior end to keep the head stationary. Use a fine minutien pin or other fine dissection tools to gently insert into the forebrain ventricle from the anterior and push downward to separate the right and left halves of the head from each other. Repeat this while moving posteriorly through the midbrain and into the hindbrain ventricle, essentially fileting the head down the midline. This minimizes manual manipulation of the eye and surrounding tissue, thereby leaving the SOS undamaged.
7. Mount each side of the head midline down, eye up. Position four posts of vacuum grease at the corners (an appropriate distance apart for the coverslip being used) and cover with a glass coverslip, pushing down sequentially on each post until the coverslip makes contact with the samples. Pipette 70% glycerol at the edge of the coverslip so that the glycerol is pulled underneath, filling the space between the coverslip and the slide.
8. Image samples within a day, or seal around the coverslip with nail polish and image samples only after the nail polish has dried. Store in the dark at 4 °C.

3. Protocol 3: Visualization of SOS using eGFP-CAAX mRNA

Synthesis of eGFP-CAAX mRNA
1. Linearize 1 µg of pCS2-eGFP-CAAX plasmid¹⁶ with NotI in a reaction volume of 40 µL for 4 hours at 37 °C.
2. To stop the restriction digest reaction, add 10 µL RNase-free water, 2.5 µL 10% SDS and 2.0 µL 10 mg/mL Proteinase K.
3. Incubate 1 hour at 50 °C.
4. Add the following to the reaction (total volume 200 µL) and proceed to next step: 50 µL RNase-free water, 20 µL 3 M sodium acetate pH 5.2 and 75.5 µL RNase-free water
  NOTE: RNase-free water is added in two separate occasions to prevent excessive dilution of the sodium acetate.
Purification of DNA through phenol/chloroform extraction and ethanol precipitation
1. Add 200 µL phenol:chloroform:isoamyl alcohol and vortex for 20 s. Separate the aqueous and organic phases through centrifugation at 18,000 x g for 5 min.
2. Transfer the upper aqueous layer to a new microcentrifuge tube, making sure to avoid the transfer of the bottom organic layer. Add an equal volume of chloroform to the new tube.
  NOTE: Addition of chloroform is optional, but it is recommended to ensure complete removal of phenol from the sample.
3. Vortex for 20 s. Separate the aqueous and organic phases through centrifugation at 18,000 x g for 5 min.
4. As before, transfer the upper aqueous layer to a new microcentrifuge tube, making sure to avoid the transfer of the bottom organic layer.
5. Add 1/10 volume of 3 M sodium acetate pH 5.2.
6. Precipitate DNA by adding 3 volumes of 100% RNase-free ethanol and chill at -20 °C for 15 min. Centrifuge at 18,000 x g for 20 min at 4 °C. A pellet should be visible. Decant the supernatant.
7. Wash the pellet with 100 µL of cold 70% ethanol/RNase-free water. After gently mixing to break the pellet loose, centrifuge at 18,000 x g for 15 min at 4 °C. A pellet should be visible. Decant the supernatant.
8. Air-dry the pellet for 5 min and resuspend the DNA in 7 µL water.
  NOTE: The pellet may need to be dried for longer than 5 min depending on the airflow available.
Transcription and purification of eGFP-CAAX mRNA
1. In an RNase-free manner, prepare an in vitro transcription reaction with a commercially available Sp6 RNA polymerase kit, using about 1 µg of purified linearized plasmid DNA obtained in Step 3.2. Incubate for 2 h at 37 °C.
  NOTE: Sp6 RNA polymerase must be used for the production of capped mRNA.
2. Add 1 µL of DNase (2 U/µL; RNase free) and incubate for 30 min at 37 °C.
3. Purify the mRNA with any commercially available RNA purification kit. Aliquot the mRNA to avoid repeated freeze-thaw, and store at -80 °C.
Injection and visualization
1. Obtain embryos as outlined in Protocol 1.1.
2. Using a microinjection apparatus, inject 300 pg of eGFP-CAAX mRNA at the 1-cell stage.
3. Screen for embryos with the bright expression of eGFP in the eyes using a fluorescence stereoscope.
4. Image the embryos as described in Protocol 1.2.
5. Alternatively, dechorionate and fix the embryos at the desired timepoint in 4% PFA for 4 hours at room temperature or overnight at 4°C. Wash the embryos in 1x PBST for 5 min, four times, and dechorionate, if not previously done. Dissect the eyes and mount them on slides as described in Protocol 2.3.

Wyniki

The zebrafish SOS appears at 20 hpf in the presumptive dorsal retina⁸. By 23 hpf the SOS transitions from its initial narrow architecture to a wide indentation and by 26 hpf it is no longer visible⁸. Therefore, to examine the SOS during normal zebrafish eye development, the embryos must be observed between 20-23 hpf. During this period, the SOS is observable through the dissecting microscope and via DIC imaging as a thin line in the dorsal e...

Dyskusje

Here, we present a standardized series of protocols to observe the SOS in the developing zebrafish embryo. To determine closure delay phenotypes, our protocols have focused on the ability to distinguish the separation of two discrete lobes of the dorsal-nasal and dorsal-temporal sides of the eye, similar to techniques used to visualize choroid fissure closure delay phenotypes in the ventral eye.

These visualization techniques can be used in conjunction with a variety of genetic manipulation te...

Ujawnienia

The authors have no conflicting interests to declare.

Podziękowania

This work was supported by Canadian Institutes of Health Research (CIHR), Natural Sciences and Engineering Research Council (NSERC), Alberta Innovates Technology Futures, and Women and Children's Health Research Institute (WCHRI).

Materiały

Name	Company	Catalog Number	Comments
1-phenyl 2-thiourea	Sigma Aldrich	P7629-10G
100 mm Petri dish	Fisher Scientific	FB0875713
35 mm Petri dish	Corning	CLS430588
Agarose	BioShop Canada Inc.	AGA001.1
Bovine serum albumin	Sigma Aldrich	A7906-100G
DIC/Fluorescence microscope	Zeiss	AxioImager Z1
Dissection microscope	Olympus	SZX12
Dissection microscope camera	Qimaging	MicroPublisher 5.0 RTV
Dow Corning High-vacuum grease	Fisher Scientific	14-635-5D
Ethyl 3-aminobenzoate methanesulfonate salt (Tricaine)	Sigma Aldrich	A5040-25G
Goat anti-rabbit Alexa Fluor 488	Abcam	ab150077
Goat serum	Sigma Aldrich	G9023
Image capture software	Zeiss	ZEN
Incubator	VWR	Model 1545
Microscope Cover Glass (22 mm x 22 mm)	Fisher Scientific	12-542B
Microscope slide	Fisher Scientific	12-544-2
Minutien pin	Fine Science Tools	26002-10
mMessage mMachine Sp6 Transcription Kit	Invitrogen	AM1340
NotI	New England Biolabs	R0189S
Paraformaldehyde (PFA)	Sigma Aldrich	P6148-500G
Phenol:Chloroform:Isoamyl Alcohol pH 6.7 +/- 0.2	Fisher Scientific	BP1752-100
Proteinase K	Sigma Aldrich	P4850
Rabbit anti-laminin antibody	Millipore Sigma	L9393
TURBO Dnase (2 U/µL)	Invitrogen	AM2238
Ultrapure low-melting point agarose	Invitrogen	16520-100
UltraPure Sodium Dodecyl Sulfate (SDS)	Invitrogen	15525017

Odniesienia

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