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Preparation of Cancer Spheroid Blocks by Flash Freezing: A Procedure To Preserve Cancer Spheroids in Frozen Matrix Blocks

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Overview

Cancer spheroids are three-dimensional aggregates of tumor cells that can be embedded in a collagen matrix. This article outlines the procedure for flash-freezing spheroid blocks to preserve their structure for histological analysis.

Key Study Components

Area of Science

  • Neuroscience
  • Cell Biology
  • Histology

Background

  • Cancer spheroids mimic in vivo tumor environments.
  • Embedding in collagen helps maintain structural integrity.
  • Flash-freezing is crucial for preserving cellular details.
  • Histological analysis requires careful preparation of samples.

Purpose of Study

  • To demonstrate the method for preparing cancer spheroids for analysis.
  • To ensure spheroid integrity during freezing.
  • To facilitate future histological studies of tumor cells.

Methods Used

  • Embedding spheroids in collagen gel.
  • Using fixative solutions to cross-link proteins.
  • Flash-freezing in liquid nitrogen.
  • Storing samples at low temperatures for analysis.

Main Results

  • The method effectively preserves spheroid structure.
  • Rapid freezing prevents ice crystal formation.
  • Samples remain viable for histological examination.
  • Embedding medium solidifies around spheroids without damage.

Conclusions

  • Flash-freezing is a reliable technique for spheroid preservation.
  • Proper embedding enhances the quality of histological samples.
  • This method can be applied to various cancer research studies.

Frequently Asked Questions

What are cancer spheroids?
Cancer spheroids are three-dimensional aggregates of tumor cells that better mimic the in vivo tumor environment compared to traditional two-dimensional cultures.
Why is flash-freezing important?
Flash-freezing preserves the structural integrity of spheroids and prevents the formation of large ice crystals that can damage cellular structures.
What is the role of collagen in this process?
Collagen provides a supportive matrix that helps maintain the shape and integrity of the spheroids during freezing and subsequent analysis.
How are the spheroids prepared for histological analysis?
Spheroids are embedded in a collagen gel, fixed with a solution, and then flash-frozen for preservation before histological examination.
What temperature should the samples be stored at?
Samples should be stored at minus 80 degrees Celsius to maintain their viability for future analysis.

Cancer spheroids are three-dimensional cellular aggregates of tumor cells. These spheroids can be embedded in the collagen matrix, resulting in the formation of spheroid blocks. To flash-freeze a spheroid block, begin by placing a collagen gel spheroid block in the center of a histology mold.

Rinse the block with a suitable buffer and supplement the mold with a fixative solution. Incubate to allow this solution to penetrate the spheroids and cross-link the cellular proteins. This step helps maintain the spheroid structure for the subsequent procedure. Next, aspirate the fixative solution.

Place the spheroid gel block into a fresh histology mold containing a thin layer of embedding medium. Overlay it with more embedding medium to completely submerge the spheroid block. Finally, submerge the mold in a liquid nitrogen bath for a short duration.

Rapid freezing prevents the formation of bigger ice crystals within spheroids. It helps in retaining spheroid integrity without causing mechanical damage. Once the embedding medium layer solidifies around the spheroid block, remove the frozen block from the mold. Store the frozen spheroid block at low temperatures for further histological analysis.

First, use small forceps to lift the block of collagen gel and spheroids from the chamber slide. Then, place the collagen gel block in a plastic histology mold. Rinse the collagen gel block with 1X PBS briefly and fix it with 4% PFA in PBS for 30 minutes at room temperature. After this, wash the collagen gel block with 1.5 milliliters of 1X PBS on a shaker for 15 minutes.

Apply a thin layer of OCT compound to the bottom of a new plastic histology mold. Then, place the fixed and washed collagen gel block on top of the OCT compound before carefully filling the rest of the mold with OCT compound. Keep the mold at 4 degrees Celsius for 1 hour. After this, flash-freeze the mold on a 100-millimeter Petri dish floating on liquid nitrogen, and store the samples at minus 80 degrees Celsius.

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