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All procedures involving human participants have been performed in compliance with the institutional, national and international guidelines for human welfare and have been reviewed by the local institutional review board.
1. Running the Assay
NOTE: Do not let sections dry out between the incubation steps.
<ol>
	<li>Hybridization of the HPV probe 
	NOTE: Ensure the probes are prewarmed to dissolve any precipitation prior to use. For this step, instead of HPV probe, peptidyl-prolyl isomerase B (PPIB) for positive control or dihydrodipicolinate reductase (DAPB) for negative control (see the Table of Materials) may also be used.
	<ol>
		<li>Tap and/or flick the slides to remove any excess liquid and place them in the slide rack. Add ~4 drops of HPV probe to entirely cover each section.</li>
		<li>Cover the tray with a lid and insert it into the oven for 2 h at 40 &#176;C. 
		NOTE: To prevent evaporation, make sure the turn knob is completely turned to the lock position.</li>
		<li>Remove the tray from the oven and remove the slide rack.</li>
		<li>One slide at a time, quickly remove any excess liquid and place the slide in a slide rack submerged in a staining dish filled with 1x wash buffer.</li>
		<li>Wash the slides in 1x wash buffer for 2 min at room temperature with constant agitation. Repeat this with fresh 1x wash buffer.</li>
	</ol>
	</li>
	<li>Hybridization of AMP1, AMP2, AMP3, and AMP4 
	NOTE: These steps include hybridization in the hybridization oven and AMP1&#8211;AMP4 from the purchased kit (see the Table of Materials).
	<ol>
		<li>Tap and/or flick to remove any excess liquid from the slides and place them in the slide rack. Add ~4 drops of AMP1 to entirely cover each section.</li>
		<li>Cover the tray with a lid and insert it into the oven for 30 min at 40 &#176;C.</li>
		<li>Remove the tray from the oven and remove the slide rack.</li>
		<li>One slide at a time, quickly remove any excess liquid and place the slide in a slide rack submerged in a staining dish filled with 1x wash buffer.</li>
		<li>Wash the slides in 1x wash buffer for 2 min at room temperature with constant agitation. Repeat this with fresh 1x wash buffer.</li>
		<li>Repeat steps 1.2.1&#8211;1.2.5, but use ~4 drops of&#160;AMP2&#160;instead of AMP1 and incubate for&#160;15 min&#160;at&#160;40 &#176;C.&#160;Wash the slides 2x for 2 min, both times in fresh wash buffer.</li>
		<li>Repeat steps 1.2.1&#8211;1.2.5, but use ~4 drops of&#160;AMP3&#160;instead of AMP1 and incubate for&#160;30 min&#160;at&#160;40 &#176;C.&#160;Wash the slides 2x for 2 min, both times in fresh wash buffer.</li>
		<li>Repeat steps 1.2.1&#8211;1.2.5, but use ~4 drops of&#160;AMP4&#160;instead of AMP1 and incubate for&#160;15 min&#160;at&#160;40 &#176;C.&#160;Wash the slides 2x for 2 min, both times in fresh wash buffer.</li>
	</ol>
	</li>
	<li>Hybridization of AMP5 and AMP6 
	&#8203;NOTE: These steps do not include hybridization in the oven but hybridization at room temperature. AMP5 and AMP6 come from the purchased kit (see the&#160;Table of Materials).
	<ol>
		<li>Tap and/or flick the slides to remove any excess liquid and place them in the slide rack. Add ~4 drops of&#160;AMP5&#160;to entirely cover each section.</li>
		<li>Cover the tray with a lid and incubate for&#160;30 min&#160;at&#160;room temperature.</li>
		<li>One slide at a time, quickly remove any excess liquid and place it in a slide rack submerged in a staining dish filled with 1x wash buffer.</li>
		<li>Wash the slides in 1x wash buffer for 2 min at room temperature with constant agitation. Repeat this with fresh 1x wash buffer.</li>
		<li>Repeat steps 1.3.1&#8211;1.3.4, but use ~4 drops of&#160;AMP6&#160;instead of AMP5 and incubate for&#160;15 min&#160;at&#160;room temperature.&#160;Wash the slides 2x for 2 min, both times in fresh wash buffer.</li>
	</ol>
	</li>
</ol>

<table><tbody><tr><td>HybEZ Oven (110v)&amp;nbsp;</td><td>Advanced Cell Diagnostics Inc.&amp;nbsp;</td><td>321710</td><td></td></tr><tr><td>HybEZ slide rack&amp;nbsp;</td><td>Advanced Cell Diagnostics Inc.&amp;nbsp;</td><td>300104</td><td></td></tr><tr><td>RNAscope 2.5 HD Detection Reagents-BROWN</td><td>Advanced Cell Diagnostics Inc.</td><td>322310</td><td>This kit includes amplification reagents AMP1, AMP2, AMP3, AMP4, AMP5 and AMP6, and detection reagents DAB-A and DAB-B</td></tr><tr><td>RNAscope 3-Plex Negative Control Probe&amp;nbsp;</td><td>Advanced Cell Diagnostics Inc.</td><td>320871</td><td>DAPB</td></tr><tr><td>RNAscope 3-Plex Positive Control Probe&amp;nbsp;&amp;nbsp;</td><td>Advanced Cell Diagnostics Inc.</td><td>320861</td><td>PPIB</td></tr><tr><td>RNAscope Probe- HPV16/18&amp;nbsp;</td><td>Advanced Cell Diagnostics Inc.</td><td>311121</td><td></td></tr><tr><td>RNAscope Wash Buffer Reagents</td><td>Advanced Cell Diagnostics Inc.</td><td>310091</td><td>Wash Buffer 50X x4</td></tr></tbody></table>

probe hybridization and signal amplification in rna in situ hybridization: a technique for detecting specific rna sequences in tissue sections

Source: Outh-Gauer, S. et al. <a href="https://www.jove.com/video/59422" target="_blank">Chromogenic In Situ Hybridization as a Tool for HPV-Related Head and Neck Cancer Diagnosis.</a> J. Vis. Exp. (2019)
This video describes a sequential hybridization strategy that involves hybridizing mRNA probes to specific target mRNA. Following probe hybridization, signal amplification is performed to enhance resolution via reduction of signal-to-noise ratio during RNA-CISH of histological samples.

Probe Hybridization and Signal Amplification in RNA In Situ Hybridization: A Technique for Detecting Specific RNA Sequences in Tissue Sections

Source: Outh-Gauer, S. et al. Chromogenic In Situ Hybridization as a Tool for HPV-Related Head and Neck Cancer Diagnosis. J. Vis. Exp. (2019)
This video ...

To detect a specific RNA sequence in a cell, begin by taking a tissue section on a glass slide. Overlay the tissue section with a suitable hybridization buffer containing the target RNA probes.
These probes are Z-shaped RNA molecules having a target recognition portion at one end and a tail sequence at another end. A spacer arm links these two ends.
Now, incubate the slide in a hybridization oven at an optimum temperature. Z-shaped RNA probes enter the cell and hybridize with the corresponding target mRNA sequence in pairs.
Remove the slide from the oven. Immerse the slide in a washing solution to remove any unbound probes and excess hybridization buffer.
Thereafter, add a pre-amplifier solution and incubate. The pre-amplifier molecule attaches to the tail sequence of two adjacent Z probes. This molecule does not bind to a single Z probe, ensuring specificity.
Next, add the amplifier reagent mixture and incubate. Multiple amplifier molecules hybridize to the single pre-amplifier sequence.
Finally, label the tissue section with the desired labeling probes to detect the presence of a specific RNA sequence in the cell.

probe-hybridization-signal-amplification-rna-situ-hybridization

Research

JoVE Encyclopedia of Experiments

Cancer Research

Head and Neck Cancer

Assays & techniques

1.0K 조회수. 출처: Outh-Gauer, S. et al. HPV 관련 두경부암 진단을 위한 도구로서의 발색성 현장 혼성화. J. Vis. 특급 (2019년) 이 동영상은 mRNA 프로브를 특정 타겟 mRNA에 하이브리드화하는 것과 관련된 순차적 하이브리드화 전략을 설명합니다. 프로브 하이브리드화 후, 조직학적 샘플의 RNA-CISH 동안 신호 대 잡음비의 감소를 통해 분해능을 향상시키기 위해 신호 증폭이 수행됩니다. 

비디오: RNA In Situ Hybridization에서 프로브 혼성화 및 신호 증폭: 조직 절편에서 특정 RNA 염기서열을 검출하는 기법 - 개념

RNAscope for In situ Detection of Transcriptionally Active Human Papillomavirus in Head and Neck Squamous Cell Carcinoma

The &#39;gold standard&#39; for oncogenic HPV detection is the demonstration of transcriptionally active high-risk HPV in tumor tissue. However, detection of E6/E7 mRNA by quantitative reverse transcription polymerase chain reaction (qRT-PCR) requires RNA extraction which destroys the tumor tissue context critical for morphological correlation and has been difficult to be adopted in routine clinical practice. Our recently developed RNA in situ hybridization technology, RNAscope, permits direct visualization of RNA in formalin-fixed, paraffin-embedded (FFPE) tissue with single molecule sensitivity and single cell resolution, which enables highly sensitive and specific in situ analysis of any RNA biomarker in routine clinical specimens. The RNAscope HPV assay was designed to detect the E6/E7 mRNA of seven high-risk HPV genotypes (HPV16, 18, 31, 33, 35, 52, and 58) using a pool of genotype-specific probes. It has demonstrated excellent sensitivity and specificity against the current &#39;gold standard&#39; method of detecting E6/E7 mRNA by qRT-PCR. HPV status determined by RNAscope is strongly prognostic of clinical outcome in oropharyngeal cancer patients.

RNAscope for In situ Detection of Transcriptionally Active Human Papillomavirus in Head and Neck Squamous Cell Carcinoma

The presence of high-risk HPV in head and neck tumor tissue is associated with favorable outcomes. The recently developed RNA in situ hybridization technique called RNAscope allows direct visualization of HPV E6/E7 mRNA in FFPE tissue sections.

에 RNAscope<em&gt; 현장에서</em&gt; 헤드 전사적으로 활동 인간 Papillomavirus의 탐지와 목 편평​​ 상피 세포 암

The &#39;gold standard&#39; for oncogenic HPV detection is the demonstration of transcriptionally active high-risk HPV in tumor tissue. However, detection ...

연구

JoVE Journal

의학

Whole-Mount In Situ Hybridization in Zebrafish Embryos and Tube Formation Assay in iPSC-ECs to Study the Role of Endoglin in Vascular Development

Vascular development is determined by the sequential expression of specific genes, which can be studied by performing in situ hybridization assays in zebrafish during different developmental stages. To investigate the role of endoglin(eng) in vessel formation during the development of hereditary hemorrhagic telangiectasia&#160;(HHT), morpholino-mediated targeted knockdown of eng in zebrafish are used to study its temporal expression and associated functions. Here, whole-mount in situ RNA hybridization (WISH) is employed for the analysis of eng and its downstream genes in zebrafish embryos. Also, tube formation assays are performed in HHT patient-derived induced pluripotent stem cell-differentiated&#160;endothelial cells (iPSC-ECs; with eng mutations). A specific signal amplifying system using the whole amount In Situ Hybridization &#8211; WISH provides higher resolution and lower background results compared to traditional methods. To obtain a better signal, the post-fixation time is adjusted to 30 min after probe hybridization. Because fluorescence staining is not sensitive in zebrafish embryos, it is replaced with diaminobezidine (DAB) staining here. In this protocol, HHT&#160;patient-derived iPSC lines containing an eng mutation are differentiated into endothelial cells. After coating a plate with basement membrane matrix for 30 min at 37 &#176;C, iPSC-ECs are seeded as a monolayer into wells and kept at 37 &#176;C for 3 h. Then, the tube length and number of branches are calculated using microscopic images. Thus, with this improved WISH protocol, it is shown that reduced eng expression affects endothelial progenitor formation in zebrafish embryos. This is further confirmed by tube formation assays using iPSC-ECs derived from a patient with HHT. These assays confirm the role for eng in early vascular development.

Presented here is a protocol for whole-mount in situ RNA hybridization analysis in zebrafish and tube formation assay in patient-derived induced pluripotent stem cell-derived endothelial cells to study the role of endoglin in vascular formation.

혈관 발달에서 엔도글린의 역할을 연구하기 위해 iPSC-ECs의 제브라피시 배아 및 튜브 형성 분석에서 시투 혼성화에 대한 전체 마운트

Vascular development is determined by the sequential expression of specific genes, which can be studied by performing in situ hybridization assays in ...

발생학

Detection of Axonally Localized mRNAs in Brain Sections Using High-Resolution In Situ Hybridization

mRNAs are frequently localized to vertebrate axons and their local translation is required for axon pathfinding or branching during development and for maintenance, repair or neurodegeneration in postdevelopmental periods. High throughput analyses have recently revealed that axons have a more dynamic and complex transcriptome than previously expected. These analysis, however have been mostly done in cultured neurons where axons can be isolated from the somato-dendritic compartments. It is virtually impossible to achieve such isolation in whole tissues in vivo. Thus, in order to verify the recruitment of mRNAs and their functional relevance in a whole animal, transcriptome analyses should ideally be combined with techniques that allow the visualization of mRNAs in situ. Recently, novel ISH technologies that detect RNAs at a single-molecule level have been developed. This is especially important when analyzing the subcellular localization of mRNA, since localized RNAs are typically found at low levels. Here we describe two protocols for the detection of axonally-localized mRNAs using a novel ultrasensitive RNA ISH technology. We have combined RNAscope ISH with axonal counterstain using fluorescence immunohistochemistry or histological dyes to verify the recruitment of Atf4 mRNA to axons in vivo in the mature mouse and human brains.

Detection of Axonally Localized mRNAs in Brain Sections Using High-Resolution In Situ Hybridization

RNA in situ hybridization (ISH) enables the visualization of RNAs in cells and tissues. Here we show how combination of RNAscope ISH with immunohistochemistry or histological dyes can be successfully used to detect mRNAs localized to axons in sections of mouse and human brains.

고해상도를 사용하여 뇌 섹션에서 Axonally 지역화 된 mRNA를 검출<em&gt; 현장에서</em&gt; 하이브리드

mRNAs are frequently localized to vertebrate axons and their local translation is required for axon pathfinding or branching during development and for ...

Probe Hybridization and Signal Amplification in RNA In Situ Hybridization: A Technique for Detecting Specific RNA Sequences in Tissue Sections

내레이션 대본

Probe Hybridization and Signal Amplification in RNA In Situ Hybridization: A Technique for Detecting Specific RNA Sequences in Tissue Sections