617.1 URMC HTC BSL2+ Non-Inflated Fresh-Frozen Embedded Lung and Associated Tissue

Slicing and blocking procedure should be accomplished in a grossing station or fume hood with the operator taking appropriate blood and body fluid precautions

Prepare dry ice-ethanol (or isobutane) bath by covering bottom of flat ice bucket or styrofoam box with dry ice pellets.

Pour in enough 200 proof ethanol to cover the dry ice and allow to boil. Once bubbling is stable, float a flat metal pan on the ethanol.

Add more dry ice and/or ehtanol as needed to maintain rapid freezing of molds set on the metal pan.

Take care that ethanol doesn't splash over onto tissue in cryomolds.

Keep the surface of the lobes moist and cool at all times

Select lobe or partial lobes for fresh embedding and freezing

Place fresh lobe on cutting surface and section tissue into slices and further into blocks.

Our standard is approximately 1cmx 1cm x 0.5 cm thick. See sectioning diagram for lobe in 604. URMC HTC protocol.

Work quickly to avoid warming of lung tissue.

Photograph resulting tissue sections as a map of the stored blocks. Include labels in photos to record work, location of blocks and processing method applied.

Suggest alternating slices of tissue between different embedding media. For example, a slice each to i-iii, then repeat:

i.Fresh Flash Frozen Block [FFb] (not embedded in any media) - note: may not withstand long freezing period

ii.Fresh OCT Frozen Block

iii.Fresh CMC Frozen Block

In the case where only 1 lobe is received, slices are taken for Cell Dissociation, Fresh Frozen Biopsy (in cryovial) and Formalin Fixed Paraffin Embedded Samples and fresh frozen blocks in OCT with potential postfixation in paraformaldehyde.

For OCT or CMC embedding: Fill the cryomolds with a thin layer of the appropriate embedding medium

Place the tissue in their respectively labeled cryomolds and position them to allow for small amount of embedding medium around the tissue

Gently press down on the tissue with forceps in an attempt to remove as much air as possible and make sure the tissue lays flat along the bottom of the cryomold during freezing so easier to face block for sectioning

Place cryomolds containing tissue on metal pan in dry-ice ethanol bath and allow to freeze while filling the cryomold with freezing medium (OCT or CMC) to completely cover the embedded tissue.

While cryomolds are freezing, print out Freezerbondz labels for each block and place label on middle of a piece of aluminum foil along with a small biohazard sticker.

Applying the label to the foil prior to wrapping the cold blocks promotes better adhesion and reduces any warming of block while wrapping.

Once frozen, quickly wrap each corresponding block with the correctly labeled aluminum foil and return to the frozen metal pan to keep frozen until transferred to -80°C freezer

Collect wrapped cryomolds into labeled freezer bags, place in cold labeled freezer boxes and store in -80°C freezer

These tissue portions of Lung, Thymus, Spleen and Lymph Node are intended for processing for total RNA and for protein homogenates.

The tissue samples are sectioned into 0.25-1.0 cm³ portions and placed in properly Freezerbondz labeled freezer vials.

The weight of the collected tissue is recorded.

The freezer tubes containing the individual tissues are then frozen over liquid nitrogen and placed at -80⁰C for storage.

Complete worksheet and virtual freezer inventory

Correctly store photographs of grossing and blocking in Database