eoe sub articles

EoE Sub Articles

1. Scraping the Slides 

<ol>
	<li>Prepare digestion/lysis buffer with 650 mL of diethylpyrocarbonate (DEPC)-treated water, 100 mL of ethylenediaminetetraacetic acid (EDTA), 50 ml of Tris hydrochloride (Tris-HCL) 2 M pH 8.8, and 200 mL of 10% sodium dodecyl sulfate (SDS) (see Table of Materials).</li>
	<li>Fill a 1.5 mL single-use polypropylene tube with 80 &#181;L of digestion/lysis buffer (see Table of Materials).</li>
	<li>Put a clean pipette tip into the buffer.</li>
	<li>Identify cancer tissues of the tumor area most suitable for macrodissection according to the appropriate H&#38;E-stained section.</li>
	<li>Macrodissect cancer tissue based on the marked H&#38;E-stained section.
	<ol>
		<li>Take a clean razor blade and gently scrape the cancer tissue off the slide, trying to keep it in one piece so that it is easier to work with.</li>
		<li>Take the pipette tip out of a single-use polypropylene tube containing buffer and use it to transfer the scrapped tissue into the buffer vial (see Table of Materials). 
		NOTE: The wet tip should attract the tissue, which makes the transfer easier.</li>
	</ol>
	</li>
	<li>Repeat step 1.5 with the rest of the slides.</li>
	<li>After all the tissue is in the single-use polypropylene tube, use the tip to make sure the tissue is fully submerged and is not stuck to the wall of the tube.</li>
	<li>Add 20 &#181;L of a subtilisin-related serine protease to the vial and gently flick to mix (see Table of Materials).</li>
	<li>Place the vial in a 55 &#176;C heat block for at least 4 h or overnight. Make sure to slightly vortex after 2 h.</li>
</ol>

<table><tbody><tr><td>10% Sodium dodecyl sulfate (SDS)&amp;nbsp;&amp;nbsp;&amp;nbsp;&amp;nbsp;</td><td>Quality Biological</td><td>351-032-721 EA</td><td>Step 2.1.</td></tr><tr><td>DEPC-treated water&amp;nbsp;&amp;nbsp;&amp;nbsp;</td><td>Quality Biological</td><td>351-068-131</td><td>Step 2.1.</td></tr><tr><td>Ethylenediaminetetraacetic acid (EDTA)&amp;nbsp;&amp;nbsp;</td><td>Corning</td><td>46-034-CL</td><td>Step 2.1.</td></tr><tr><td>Tris hydrochloride (Tris-HCL) 2 M pH 8.8&amp;nbsp;&amp;nbsp;&amp;nbsp;</td><td>Quality Biological</td><td>351-092-101</td><td>Step 2.1.</td></tr><tr><td>Proteinase K&amp;nbsp;</td><td>New England Biolabs</td><td>P8107S&amp;nbsp;</td><td>Step 2.8.</td></tr><tr><td>Single-use polypropylene (Eppendorf) tube</td><td>Eppendorf</td><td>24533495</td><td>Step 2.5.2.</td></tr></tbody></table>

ffpe tumor tissue macrodissection: a technique to obtain specific tumorous tissue from unstained specimens

Source: Sugimoto, K. et al. <a href="https://www.jove.com/video/61355" target="_blank">Genome-Wide Analysis of DNA Methylation in Gastrointestinal Cancer.</a> J. Vis. Exp. (2020)
This video describes a method for the manual macrodissection of cancer tissue from unstained tissue specimens to obtain a specific cancer tissue. The tissue section can be processed further to obtain DNA for genome-wide studies on gastrointestinal cancers.

FFPE Tumor Tissue Macrodissection: A Technique to Obtain Specific Tumorous Tissue from Unstained Specimens

Source: Sugimoto, K. et al. Genome-Wide Analysis of DNA Methylation in Gastrointestinal Cancer. J. Vis. Exp. (2020)
This video describes a method for the ...

To begin macrodissection, take a glass slide carrying a tissue specimen. Additionally, take a reference slide carrying the same tissue specimen and stain it using hematoxylin and eosin for H&#38;E stain.
In normal cells, hematoxylin imparts a blue stain to nucleic acids, while the eosin counterstain shows the cellular proteins pink. The deep blue coloration of the nucleus helps in differentiating cancer cells from normal cells.
Overlay the H&#38;E stained slide with the unstained slide to align the tissue specimens. Locate the portion containing tumor cells on the H&#38;E stained slide. Mark the corresponding area on the unstained slide.
Scrape off the desired tissue from the unstained slide. Using a wet pipette tip, collect the scraped tissue to ensure an easy transfer of the tissue specimen. Transfer the tissue into a tube containing a lysis buffer. Components of the lysis buffer digest the tissue, releasing the constituents of the cell.
Treat the lysate with a suitable protease and incubate at a high temperature. The protease cleaves the contaminating DNases, thereby protecting the DNA from degradation. Store the DNA containing tissue lysate for downstream analysis.

ffpe-tumor-tissue-macrodissection-technique-to-obtain-specific

Research

JoVE Encyclopedia of Experiments

Cancer Research

Gastrointestinal Cancer

Assays and techniques

Vidéo: Macrodissection de tissu tumoral FFPE : une technique pour obtenir un tissu tumoral spécifique à partir d’échantillons non colorés - Concept

Laser-capture Microdissection of Human Prostatic Epithelium for RNA Analysis

The prostate gland contains a heterogeneous milieu of stromal, epithelial, neuroendocrine and immune cell types. Healthy prostate is comprised of fibromuscular stroma surrounding discrete epithelial-lined secretory lumens and a very small population of immune and neuroendocrine cells. In contrast, areas of prostate cancer have increased dysplastic luminal epithelium with greatly reduced or absent stromal population. Given the profound difference between stromal and epithelial cell types, it is imperative to separate the cell types for any type of downstream molecular analysis. Despite this knowledge, the bulk of gene expression studies compare benign prostate to cancer without micro-dissection, leading to stromal bias in the benign samples. Laser-capture micro-dissection (LCM) is an effective method to physically separate different cell types from a specimen section. The goal of this protocol is to show that RNA can be successfully isolated from LCM-collected human prostatic epithelium and used for downstream gene expression studies such as RT-qPCR and RNAseq.

The goal of this protocol is to use laser-capture micro-dissection as an effective method to isolate pure populations of cell types from heterogeneous prostate tissues for downstream RNA analysis.

Laser-microdissection de la prostate humaine épithélium pour l&#39;analyse de l&#39;ARN

The prostate gland contains a heterogeneous milieu of stromal, epithelial, neuroendocrine and immune cell types.  Healthy prostate is comprised of ...

Recherche

JoVE Journal

Médecine

SIVQ-LCM Protocol for the ArcturusXT Instrument

SIVQ-LCM is a new methodology that automates and streamlines the more traditional, user-dependent laser dissection process.&#160;It aims to create an advanced, rapidly customizable laser dissection platform technology. In this report, we describe the integration of the image analysis software Spatially Invariant Vector Quantization (SIVQ) onto the ArcturusXT instrument. The ArcturusXT system contains both an infrared (IR) and ultraviolet (UV) laser, allowing for specific cell or large area dissections. The principal goal is to improve the speed, accuracy, and reproducibility of the laser dissection to increase sample throughput. This novel approach facilitates microdissection of both animal and human tissues in research and clinical workflows.

SIVQ-LCM is an innovative approach that harnesses a computer algorithm, Spatially Invariant Vector Quantization (SIVQ), to drive the laser capture microdissection (LCM) process. The SIVQ-LCM workflow greatly improves the speed and accuracy of microdissection, with applications in both the research and clinical settings.

Protocole SIVQ-LCM pour l&#39;instrument ArcturusXT

SIVQ-LCM is a new methodology that automates and streamlines the more traditional, user-dependent laser dissection process.&#160;It aims to create an ...

Biologie

Preparation of Formalin-fixed Paraffin-embedded Tissue Cores for both RNA and DNA Extraction

Formalin-fixed paraffin embedded tissue (FFPET) represents a valuable, well-annotated substrate for molecular investigations. The utility of FFPET in molecular analysis is complicated both by heterogeneous tissue composition and low yields when extracting nucleic acids. A literature search revealed a paucity of protocols addressing these issues, and none that showed a validated method for simultaneous extraction of RNA and DNA from regions of interest in FFPET. This method addresses both issues. Tissue specificity was achieved by mapping cancer areas of interest on microscope slides and transferring annotations onto FFPET blocks. Tissue cores were harvested from areas of interest using 0.6 mm microarray punches. Nucleic acid extraction was performed using a commercial FFPET extraction system, with modifications to homogenization, deparaffinization, and Proteinase K digestion steps to improve tissue digestion and increase nucleic acid yields. The modified protocol yields sufficient quantity and quality of nucleic acids for use in a number of downstream analyses, including a multi-analyte gene expression platform, as well as reverse transcriptase coupled real time PCR analysis of mRNA expression, and methylation-specific PCR (MSP) analysis of DNA methylation.

This modified extraction protocol improves RNA and DNA yields from more precisely targeted regions of interest in histopathologic tissue blocks.

Préparation de Cores de tissus enrobés de paraffine fixés au formol pour les ARN et d&#39;extraction d&#39;ADN

Formalin-fixed paraffin embedded tissue (FFPET) represents a valuable, well-annotated substrate for molecular investigations. The utility of FFPET in ...

FFPE Tumor Tissue Macrodissection: A Technique to Obtain Specific Tumorous Tissue from Unstained Specimens

Transcription

FFPE Tumor Tissue Macrodissection: A Technique to Obtain Specific Tumorous Tissue from Unstained Specimens