This Non-provisional application claims priority under 35 U.S.C. § 119(a) on Patent Application No(s). 106113526 filed in Taiwan, Republic of China on Apr. 21, 2017, the entire contents of which are hereby incorporated by reference.
The present disclosure relates to a method and kit for staining a neural tissue sample, which may use with X-ray microscopy for visualizing neurons.
Golgi-Cox staining is a method for staining neurons and discovered by Camillo Golgi in 1873. This method is to stain neurons by placing the neural tissue in the potassium dichromate solution and the silver nitrate solution. However, it requires the neural tissue to be immersed in the aforementioned solutions for a long time. The conventional Golgi-Cox staining is characterized in that the neurons in the neural tissue is stained with a hit rate of 1%-10%, such that the neurological morphology of the neural tissue can be seen.
Several studies have been made to modify the conventional Golgi-Cox staining method, with a limited hit rate. As shown in the study made by Anan Li et al. (Anan Li et al. (2010). Micro-optical sectioning tomography to obtain a high-resolution atlas of the mouse brain. Science, 330, 1404-8.), a whole mouse brain sample is prepared and stained by the modified Golgi-Cox staining method and embedded with Spurr resin. Later, the image data are acquired by the Micro-Optical Sectioning Tomography (MOST) system which is developed by the authors. Throughout data acquisition, the section thickness was 1.0·m, and an objective (40×, numerical aperture 0.8) was used for imaging. Please refer to
In addition to the long-term staining, the existing Golgi-Cox staining methods may have difficulty to present a reconstructed 3D image which has an actual neuroanatomical connectivity of the nerve system because of their low hit rates (1%-10%). In detailed, as discussed as above, because only 1% to 10% of neurons are stained by the existing Golgi-Cox staining methods, when a certain neuron is shown to be not connected with other neurons, it is not sure that there are actually no such neurons that are connected with it. Or, there are such neurons, but they are just not shown because of not being stained. Hence, even with a high-resolution 3D imaging system, a precise neuroanatomical connectivity is still unavailable when a conventional Golgi-Cox staining method is used.
Hence, it has become an urgent need to provide a method and kit for staining a neural tissue sample, without long-term staining but with an elevated hit rate, to be able to observe the detailed morphology of the neural tissue under a high-resolution X-ray microscope.
According to an objective of the present disclosure, a method and kit for staining neural tissue sample with an elevated hit rate but without long-term staining are provided. This method and kit can be used with the high-resolution X-ray microscopy to observe the detailed neural morphology and the neuroanatomical connectivity of the neural tissue sample.
The present disclosure provides a method for staining a neural tissue sample. The method comprises the following steps: placing a neural tissue sample in an acrolein solution in the dark for fixation; placing the fixed neural tissue sample in a Golgi-Cox solution in the dark; replacing the Golgi-Cox solution; incubating the neural tissue sample placed in the replaced Golgi-Cox solution at a temperature ranging from 36° C. to 38° C.; gradiently dehydrating the neural tissue sample; and embedding the dehydrated neural tissue sample with Petropoxy 154 resin.
In one embodiment, the neural tissue sample is a whole brain sample.
In one embodiment, the acrolein solution is a 4%-10% acrolein solution.
In one embodiment, the Golgi-Cox solution is replaced twice in the step of replacing the Golgi-Cox solution.
In one embodiment, the Golgi-Cox solution is replaced every 2 to 5 days in the step of replacing the Golgi-Cox solution.
In one embodiment, the neural tissue sample is gradiently dehydrated by alcohol in the step of gradiently dehydrating the neural tissue sample.
In one embodiment, the neural tissue sample is gradiently dehydrated by a 50%, 75%, 95%, and 100% alcohol solution in the step of gradiently dehydrating the neural tissue sample.
In one embodiment, before performing the step of gradiently dehydrating the neural tissue sample, the method further comprises the step of sectioning the neural tissue sample after the neural tissue sample is undergone being placed in the Golgi-Cox solution.
The present disclosure further provides a method for visualizing neurons which comprises the following steps: staining a neural tissue sample using the above mentioned method to obtain the embedded neural tissue sample; and performing data acquisition and image reconstruction on the neural tissue sample using X-ray microscopy.
The present disclosure further provides a kit for staining a neural tissue sample. The kit comprises an acrolein solution, a Golgi-Cox solution, and Petropoxy 154 resin.
In one embodiment, the acrolein solution is a 4%-10% acrolein solution.
In one embodiment, the Golgi-Cox solution comprises a 5% aqueous potassium dichromate solution, a 5% aqueous mercury chloride solution, a 5% aqueous potassium chromate solution and water in a volumetric ratio of 5:5:4:10, respectively.
In one embodiment, the kit further comprises an alcohol solution for dehydrating the neural tissue sample.
In one embodiment, the concentration of the alcohol solution ranges from 50% to 100%.
Accordingly, the method and kit for staining a neural tissue sample use the acrolein solution for fixation, use the Golgi-Cox solution for sample staining and thermal staining, and use Petropoxy 154 resin for embedding the dehydrated neural tissue sample, and have an elevated hit rate but without long-term staining. The method and kit may also be used with high-resolution X-ray microscopy to observe the detailed morphology and the neuroanatomical connectivity of the neural tissue sample.
The invention will become more fully understood from the detailed description and accompanying drawings, which are given for illustration only, and thus are not limitative of the present invention, and wherein:
The embodiments of the invention will be apparent from the following detailed description, which proceeds with reference to the accompanying drawings, wherein the same references relate to the same elements.
In the present embodiment, the neural tissue sample can be a whole brain sample obtained from a mouse. The obtained neural tissue sample is placed in the acrolein solution for tissue fixation, such that the original cellular and tissue morphology and structure of the neural tissue sample can be maintained as much as possible. The acrolein solution can be diluted in the PBS (phosphate buffered saline) buffer, and is preferable a 4% to 10% (v/v) acrolein solution diluted in the PBS buffer.
After fixation, the fixed neural tissue sample is placed in the Golgi-Cox solution in the dark (step S12). In the present embodiment, the neural tissue sample is placed in the Golgi-Cox solution at room temperature in the dark, and the Golgi-Cox solution comprises a 5% (w/v) aqueous potassium dichromate solution, a 5% (w/v) aqueous mercury chloride solution, a 5% (w/v) aqueous potassium chromate solution and water in a volumetric ratio of 5:5:4:10, respectively.
Later, the Golgi-Cox solution is replaced (step S13). The replacement of the Golgi-Cox solution means to replace the used solution with a fresh Golgi-Cox solution. The replacing times (i.e., how many times the solution are replaced) and the replacing interval are not limited herein. In the present embodiment, the Golgi-Cox solution can be replaced twice. The first replacement is to replace the Golgi-Cox solution used in the step S12 with a fresh Golgi-Cox solution, two days after the fixed neural tissue sample is placed in the Golgi-Cox solution in the dark. And, the second replacement is to replace the Golgi-Cox solution used in the first replacement with another fresh Golgi-Cox solution, five days after the first replacement.
After replacing the Golgi-Cox solution, the neural tissue sample placed in the replaced Golgi-Cox solution is incubated at a temperature ranging from 36° C. to 38° C. (step S14), which is a step of thermal staining. In the present embodiment, the neural tissue sample placed in the Golgi-Cox solution is incubated in an incubator at 37° C.
Later, the neural tissue sample is gradiently dehydrated (step S15). The gradient dehydration can be carried out with alcohol solutions serially diluted to various concentrations. In details, the neural tissue sample is sequentially placed into the alcohol solutions with different concentrations, from low to high, to prevent the neural tissue sample from deformation resulted from acute dehydration. In the present embodiment, the neural tissue sample can be gradiently dehydrated with 50% (v/v), 75% (v/v), 95% (v/v), and 100% (v/v) aqueous alcohol solutions.
After the neural tissue sample is gradiently dehydrated, it can be embedded in Petropoxy 154 resin (step S16). In this step, the Petropoxy 154 resin is used for coloring and embedding. In the present embodiment, the gradiently dehydrated whole mouse brain (i.e. the neural tissue sample) which is fixed by the acrolein solution and stained and thermally stained by the Golgi-Cox solution can be embedded and colored with the Petropoxy 154 resin. For example, the Petropoxy 154 resin can be 100% Petropoxy 154 resin, and preferably 90% (v/v) Petropoxy 154 resin which is composed of 90% of Petropoxy 154 resin and 10% of 99.5% pure ethanol. Such concentration may facilitate the Petropoxy 154 resin to infiltrate into the tissue.
The present disclosure further provides a reagent kit for staining a neural tissue sample. The reagent kit comprises an acrolein solution, a Golgi-Cox solution and Petropoxy 154 resin. In one embodiment, the acrolein solution can be diluted to 4% (v/v) to 10% (v/v) with a PBS buffer. The Golgi-Cox solution can comprises a 5% (w/v) aqueous potassium dichromate solution, a 5% (w/v) aqueous mercury chloride solution, a 5% (w/v) aqueous potassium chromate solution and water, in a volumetric ratio of 5:5:4:10, respectively. In addition, the reagent kit for staining the neural tissue sample may further comprises a solution for gradiently dehydrating the neural tissue sample, such as an alcohol solution. In the present disclosure, the category of the reagent for gradiently dehydration is not limited, and the category of such reagent can comprises a variety of solutions which can gradiently dehydrate the tissue sample. Such reagent can be the solutions of the same type and with serially increased concentrations. In one embodiment, the solution for gradiently dehydrating the neural tissue sample can be the alcohol solutions with concentrations of 50% (v/v), 75% (v/v), 95% (v/v) and 100%.
In summary, the method and kit for staining a neural tissue sample utilize the acrolein solution for fixation, utilize the Golgi-Cox solution for sample staining and thermal staining, and use Petropoxy 154 resin for embedding the dehydrated neural tissue sample, and have an increased hit rate but without long-term staining. The method and kit may also be used with high-resolution X-ray microscopy to observe the detailed morphology and the neuroanatomical connectivity of the neural tissue sample.
In the following experimental examples, the practicing steps and functions of the method and kit for staining the neural tissue sample and the method for visualizing neurons are shown. It should be noted that the following examples are used to describe some practicing details so as to enable those skilled in the art to perform and/or use the method and kit disclosed by this disclosure, and they are not used to limit the scope of the present invention.
A Golgi-Cox solution comprised a 5% (w/v) aqueous potassium dichromate solution, a 5% (w/v) aqueous mercury chloride solution, a 5% (w/v) aqueous potassium chromate solution and water in a volumetric ratio of 5:5:4:10, respectively. Firstly, it was to prepare a solution A, solution B and solution C. The solution A was a 5% (w/v) aqueous potassium dichromate solution, prepared by dissolving 10 g of potassium dichromate in 200 ml of distilled water. The solution B was a 5% (w/v) aqueous mercury chloride solution, prepared by dissolving 10 g of mercury chloride in 200 ml of distilled water. The solution C was a 5% (w/v) aqueous potassium chromate solution, prepared by 8 g of potassium chromate in 160 ml of distilled water. The solutions A and B were mixed with each other in a 500 ml glass flask, and the solution C was mixed with 400 ml of distilled water in a 1000 ml glass flask. The mixed solution of A and B was slowly poured into the mixed solution of C and water and stirred with a glass rod simultaneously during pouring. After standing in the dark for 5 days, the supernatant of the resultant mixture was used for the following steps by aspiration (avoiding sediments).
In the present experimental example, it was to obtain and then fix neural tissue samples. The C57BL/6J mice were used in this experimental example and deeply anesthetized with sodium pentobarbital (100 mg/Kg). The brain of each mouse was removed and immersed in the 10% acrolein solution (diluted by 4% PBS buffer) and stand for overnight at 4° C. Later, the mouse brain was washed in PBS buffer for three days in the dark.
The neural tissue sample was stained and thermally stained with Golgi-Cox solution. The mouse brain was immersed in Golgi-Cox solution at room temperature and in the dark. Two days later, the Golgi-Cox solution was refreshed. On the fifth day after being immersed in the refreshed Golgi-Cox solution, the sample was replaced with another fresh Golgi-Cox solution, followed by being placed into a 37° C. incubator for thermally staining for seven days. Later, the mouse brain was washed in PBS buffer for one day: the PBS buffer was refreshed for every three hours and after the PBS buffer was refreshed twice the mouse brain was immersed in a fresh PBS buffer and stand for overnight. The washed mouse brain can be used for coloring and embedding.
The neural tissue sample prepared by the Example 3 was colored and embedded with Petropoxy 154 resin. The sample can be colored and embedded after section, or the whole brain sample can be directly colored and embedded. In this experimental example, the mouse brain sample can be sectioned at a thickness of 100 micrometers. The sections were washed with water thrice (each time for five minutes) and dehydrated through a graded series of alcohol solutions with ascending concentrations (placed in 50% (v/v) ethanol once, and then 75% (v/v) ethanol once, 95% (v/v) ethanol once, last in 100% ethanol twice). After dehydration, the sections were embedded with Petropoxy 154 resin (containing 90% Petropoxy 154 resin and 10% of 99.5% ethanol) at 70° C. overnight for curing. Alternatively, the whole mouse brain was washed in the water for overnight and then dehydrated through a graded series of alcohol solutions with ascending concentrations (placed in 50% (v/v) ethanol once, and then 75% (v/v) ethanol once, 95% (v/v) ethanol once, last in 100% ethanol twice). After dehydration, the whole mouse brain sample was embedded with Petropoxy 154 resin (containing 90% Petropoxy 154 resin and 10% of 99.5% ethanol) at 70° C. overnight for curing.
The mouse brain sample was removed according to the steps described in the Example 2 and then immersed in the formaldehyde solution for fixation. The fixed mouse brain sample was stained with Golgi-Cox solutions according to the steps described in the Example 3. In this example, the mouse brain sample was colored with lithium hydroxide (LiOH) or ammonium hydroxide (NH4OH) instead. The stained mouse brain was sectioned at a thickness of 100 micrometers. The sections were immersed in 1% (w/v) LiOH (or in 10% w/v NH4OH) until the color of the samples was become black. It took about several minutes. The sections were then washed with water thrice (each time for five minutes) and dehydrated through a graded series of alcohol solutions with ascending concentrations (placed in 50% (v/v) ethanol once, and then 75% (v/v) ethanol once, 95% (v/v) ethanol once, last in 100% ethanol twice). At last, the sections were embedded in Epon 812 resin.
The reconstructed image of a large volumetric and high-resolution (of micro-scales) was taken with X-ray tomography by using the BL01A beamline from the storage ring of the NSRRC (Taiwan National Synchrotron Radiation Research Center). The aforementioned beamline was a full-spectrum X-ray beamline. The X-ray was passed through an attenuator to reduce its intensity. After that, the X-ray was then passed through the sample and then converted to a visible light by a scintillation crystal. The visible light was then introduced into an objective and detectors through prisms.
The specimen was mount on the sample carrier. Each sample was imaged with an exposure time of 200 milliseconds (ms) on every 0.3°. After taking 600 images consecutively, those images were reconstructed by Octopus Imaging Software. The 3D image was produced by Amira.
The reconstructed image of a large volumetric and high-resolution (of nano-scales) was taken with transmission X-ray microscopy by using the BL01B beamline from the storage ring of the NSRRC (Taiwan National Synchrotron Radiation Research Center). The aforementioned beamline was an X-ray beamline with a certain wavelength. The X-ray was passed through an X-ray tube to focus. After that, the focused X-ray was then passed through a pinhole and then focused on the sample. The light which was passed through the sample was passed through a Fresnel waveband to magnify the image and then passed through a phase ring to generate a phase difference. At last, the X-ray was converted to a visible light by a scintillation crystal, magnified again by the objective, and imaged by a detector. The energy of the imaging X-ray was 8 KeV and each image was taken with an exposure time of 50 ms.
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The experimental results clearly demonstrate that the method and kit for staining the neural tissue sample and method for visualizing neurons can significantly increase the hit rate of staining neurons, and the dendrites/axons of neurons can be shown in a continuous pattern in the high-resolution reconstructed image. Hence, the connectivity of neurons can be clearly shown through processing the neural tissue sample by the method and kit provided by the present disclosure. As described above, the method and kit for staining a neural tissue sample provided by this disclosure use the acrolein solution for fixation, use the Golgi-Cox solution for sample staining and thermal staining, and use Petropoxy 154 resin for embedding the dehydrated neural tissue sample, and have an increased hit rate but without long-term staining. The method and kit may also be used with high-resolution X-ray microscopy to observe the detailed morphology and the neuroanatomical connectivity of the neural tissue sample.
Although the present invention has been described with reference to specific embodiments, this description is not meant to be construed in a limiting sense. Various modifications of the disclosed embodiments, as well as alternative embodiments, will be apparent to persons skilled in the art. It is, therefore, contemplated that the appended claims will cover all modifications that fall within the true scope of the present invention.
Number | Date | Country | Kind |
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106113526 | Apr 2017 | TW | national |