intracameral injection of trypan blue in rat eyes to assess delivery into the anterior chamber

<meta charset="utf8"></head><body>优化的大鼠前房内注射技术以减少组织损伤

The bioavailability of compounds delivered by topical administration to the surface of the eye is greatly limited, typically &#60;5%1. Compounds administered by eye drops are mainly&#160;eliminated by drainage, induced lacrimation, tear fluid turnover, and conjunctival absorption. In addition, the permeation of compounds through the ocular surface is highly restricted by the cornea-conjunctiva barrier1,2,3. The cornea is composed of three main layers: the outermost epithelium, the intermediate stroma, and the innermost endothelium. The superficial corneal epithelium is interconnected by strong&#160;tight junctions and creates high paracellular resistance, which is the main barrier to substance permeability. Multiple epithelium layers further limit the permeation of hydrophilic and large molecules through the intercellular spaces of the cornea epithelium. Succeeding the epithelium, the stroma is composed of collagen fibers and contains aqueous pores. In contrast to the corneal epithelium, the stroma allows the movement of hydrophilic drugs; however, it is greatly impermeable to lipophilic compounds1,2,3. Together, the corneal epithelium and stromal layers present major tissue barriers that limit drug absorption. The corneal endothelium is not considered to restrict drug transport.
Alternative to the corneal delivery route is the conjunctival route. The conjunctiva is a multi-epithelium layer that covers the inner side of the eyelids and the anterior part of the sclera. The conjunctiva is characterized by fewer tight junctions than the corneal epithelium, allowing better permeability of hydrophilic drugs. However, vascularization of the conjunctiva results in systemic absorption of a large fraction of the administered molecules, again greatly limiting the bioavailability of delivered compounds to the anterior chamber1,2. An efficient way to bypass the outer ocular permeability barriers is to deliver the drug directly into the region of interest. For example, intravitreal injection is common for delivery into the vitreous humor4. Likewise, intracameral injection is utilized for delivery into the anterior chamber5. Establishing an efficient concentration at the anterior chamber is critical to various clinical situations, such as the treatment of infection by intracameral injection of antibiotics and postoperative anti-inflammatory treatments in cataract surgeries. Despite the advantage of improved substance bioavailability granted by intracameral injection, there are major safety concerns that should be considered. For example, intracameral drug injection may induce increased intraocular pressure, toxic anterior segment syndrome, and toxic endothelial cell destruction syndrome5,6. It is, therefore, essential to carefully assess in pre-clinical studies the efficacy and safety of drugs delivered by intracameral injections to maximize treatment efficiency and minimize potential adverse effects in patients.
Experimental animal models are indispensable in pre-clinical studies to investigate new treatments. Small rodents, such as mice and rats, are the most commonly utilized laboratory animals for such purposes. These animals exhibit numerous similarities to human anatomy and physiology, providing valuable insights. Moreover, their use is economically advantageous due to their small size, ease of maintenance, fast gestation, and ability to produce large numbers of offspring7.
Despite the widespread use of small rodents in eye disease models, their unique eye dimensions and anatomy pose significant challenges during experimental manipulations. For instance, procedures like intracameral injections, which are relatively straightforward in humans, become technically demanding in mice and rats. The challenges stem from factors such as the small volume of aqueous humor, the relatively large and inflexible lens, and the obstructive positioning and curvature of the lens within the rodents&#39; eyes (Figure 1)8. These challenges increase the risk of damage during intracameral injections in rodents, leading to potential adverse effects and introducing experimental variability that can impact the validity of study conclusions. In our research, we have successfully developed a procedure for safe intracameral injection in rats. The technique involves creating a long, flat, self-sealing tunnel in the cornea into the anterior chamber. This method not only ensures precision but also enhances experimental reproducibility, addressing the issues associated with injection techniques in small rodents.
<img alt="Figure 1" class="xfigimg" src="/files/ftp_upload/66662/66662fig01.jpg" /> 
Figure 1: Schematic representation of the anatomical anterior segment features of rat and human eyes. <a href="https://www.jove.com/files/ftp_upload/66662/66662fig01large.jpg" target="_blank">Please click here to view a larger version of this figure.</a>

<meta charset="utf8"></head><body>作者聚焦：一种提高啮齿动物眼科精确度的前房内注射新方案

不良反应风险低的大鼠前房内注射

Intracameral injections allow to bypass the outer ocular barrier and directly deliver compounds to the aqueous humor. However, conducting intracameral injection in rodent present technical challenges that may result in adverse effect and impact the experimental outcome. We, therefore, design the protocol considering the red-eye anatomy to allow intracameral injection with minimal risk of adverse effects.Intracameral injections in rodents involve the risk of tissue damage due to the small eye dimensions, limited aqueous humor of volume, and lens position. Tissue damage during manipulation can lead to complication, like anterior chamber shallowing, lens injury, endothelial cell damage, and inflammation. All of this cause experimental variability and influence findings.The length and angle of the incision are critical. We make the incision in the central corneal area where the anterior chamber is the deepest at an angle close to flat. This generates a long tunnel, which helps in reducing the loss of aqueous humor.Injecting through the tunnel improves precision and reduces the likelihood of touching the lens. The described intracameral injection method can be utilized in various experimental settings to generate disease models or assess different treatments. We expect that the precision and reproducibility of this injection technique will be a valuable tool in experimental ophthalmology.

大鼠眼前房内注射台盼蓝以评估进入前房的输送

intracameral-injection-trypan-blue-rat-eyes-to-assess-delivery-into

Research

JoVE Journal

Biology

Intracameral Injection of Trypan Blue in Rat Eyes to Assess Delivery into the Anterior Chamber

39 次观看. 首先将 5 微升台盼蓝装入无菌 10 微升玻璃汉密尔顿注射器中，该注射器配有 34 号钝针。然后将加载的注射器针头通过自密封角膜隧道插入前房。将溶液注射到眼睛中，并将针头固定两到三秒，直到所有液体清除。轻轻拉出针头。在狭缝显微镜下检查。评估前房的深度以排除浅层，并验证前房中是否存在台盼蓝。使用该方案，将 Sprague-Dawley...

视频: 大鼠眼前房内注射台盼蓝以评估进入前房的输送

Intracameral Injection in Rats with Low Risk of Adverse Effects

Intracameral injection is a standard administration routine in ophthalmology. The application of intracameral injection in rodents for research is challenging due to the limiting dimensions and anatomy of the eye, including the small aqueous humor volume, the lens curvature, and lens thickness. Potential damage during intracameral injections introduces adverse effects and experimental variability. This protocol describes a procedure for intracameral injection in rats, allowing precision and reproducibility.
Sprague-Dawley rats were used as experimental models. Since the lens position in rats protrudes into the anterior chamber, injecting from the periphery, as done in humans, is unfavorable. Therefore, an incision is created in the central corneal region using a 31 gauge 0.8 mm stiletto blade to form a self-sealing tunnel into the anterior chamber. An incision at&#160;an angle close to the flat allows to create a long tunnel, which minimizes the loss of aqueous humor and shallowing of the anterior chamber. A 34 gauge nanoneedle is inserted into the tunnel for injection. This enables penetration with minimal friction resistance and avoids touching the lens. Injection of trypan-blue allows&#160;visualization&#160;by slit microscopy the presence of the dye in the anterior chamber and exclude leakage. Bioavailability to the corneal endothelial layer is demonstrated by injection of Hoechst dye, which stained the nuclei of corneal endothelial cells after injection.
In conclusion, this protocol implements a procedure for accurate intracameral injection in rats. This procedure may be used for intracameral delivery of various drugs and compounds in experimental rat models, increasing the efficiency and reproducibility of ophthalmic research.

This protocol describes a technique for intracameral injection in rats using a central corneal incision and a long tunnel into the anterior chamber. This injection method minimizes the risk of inducing inadvertent tissue damage and thereby improves precision and reproducibility.

Intracameral injection is a standard administration routine in ophthalmology. The application of intracameral injection in rodents for research is ...

科研

生物学

Creating a Self-Sealing Corneal Tunnel for Intracameral Injection in Rats

To begin, prepare the animal for surgery and apply 0.3%ofloxacin and 0.1%dexamethasone to the animal's eye. Using surgical ophthalmic forceps, hold the superior sclera at the vertical midline next to the corneoscleral junction to stabilize the eye. Under a surgical microscope, place a sterile 0.8 millimeter 31-gauge stiletto blade in the paracentral corneal region on the vertical midline.In this position, puncture the cornea to make an incision and create a long tunnel until it penetrates into the central area of the anterior chamber. Then apply topical 0.3%ofloxacin and 0.1%dexamethasone to the eye. Next, under a slit microscope, observe the depth of the anterior chamber of the injected eye compared to the non-injected eye.Also observe the lens of the injected eye compared to the non-injected eye.

创建用于大鼠前房内注射的自密封角膜隧道

Begin by loading five microliters of trypan blue into a sterile 10 microliter glass Hamilton syringe, equipped with a 34 gauge blunt needle. Then insert the loaded syringe needle through the self-sealing corneal tunnel into the anterior chamber. Inject the solution in the eye and hold the needle in place for two to three seconds until all fluid clears.Pull out the needle gently. Examine under slit microscopy. Evaluate the depth of the anterior chamber to exclude shallowing, and verify the presence of trypan blue in the anterior chamber.Using this protocol, the corneas of Sprague-Dawley rats were injected with trypan blue. Immediate slit lamp examination post-injection revealed that the anterior chamber was visibly stained with trypan blue, confirming the successful delivery of the substance to the target area.

Intracameral Injection of Hoechst to Assess the Bioavailability of Dye to the Corneal Endothelial Cell Layer

To begin, load five microliters of hoechst solution into a sterile 10 microliter glass Hamilton syringe, attached to a 34 gauge blunt needle. Insert this syringe needle into the anterior chamber through the self-sealing corneal tunnel, and inject the solution. Hold the needle in place for two to three seconds, until all fluid clears.Pull out the needle slowly to remove it, avoiding leakage. Next, enucleate both eyes. To isolate the corneas, cut the sclera around the optic nerve, and make four additional cuts from the optic nerve towards the cornea.Drain the excess fluid with the Whatman filter paper. Spread out the cut sclera, and separate the retina from the sclera. Pull out and discard the lens and retina.Next, remove the iris. Cut and discard the sclera around the cornea. And carefully lift up the cornea.Placing the corneas on a glass slide, stain them with 0.5%Alizarin Red to identify endothelial cells. After removing the excess stain, wash the cornea three times, and place a cover slip on it. Examine the corneas under a light microscope to image the Alizarin Red staining of endothelial cells.Also, evaluate the corneas under a fluorescent microscope to observe hoechst staining, and compare it to the non-injected cornea as control. Hoechst dye, a DNA binding cell permeable fluorescent marker, was utilized to assess drug bioavailability through intracameral injection. Corneal endothelial cell uptake of hoechst was examined 15 minutes post-injection by fluorescent microscopy.Alizarin Red staining highlighted the intercellular borders of the endothelial layer. Also, positive hoechst staining within corneal endothelial cell nuclei confirmed the successful delivery of the dye via this method.