Table 1.
Tissue preservation/stabilization variables associated with biomarker analysis
| Variables | Possible reasons | Potential solutions |
|---|---|---|
| Pre-analytical | ||
| Tissue evaluation time (grossing) |
Delay in transport | Transport and process tissues as soon as possible post excision |
| Time delay to preservation |
Heavy work load or back-log of cases | Communicate tissue processing requirements with clinical and laboratory staff |
| Phosphatase, kinase and proteinase activity in tissue |
Type of preservative/fixation | Use rapid preservative method compatible with downstream analysis |
| Lack of inhibitors/stabilization in transport medium |
Use preservative/fixative containing phosphatase, kinase, proteinase inhibitors or with inhibitor activity |
|
| Delay in transport/preservation/ stabilization |
Transport, preserve and process tissues as soon as possible post excision |
|
| Storage temperature | Store tissue at appropriate temperature for preservation solution |
|
| Introduction of phosphatases/ proteinases from the environment |
Maintain clean tissue processing/grossing areas | |
| Degree of fixative cross- linking |
Preservative/fixative containing formalin, gluteraldehyde or other cross-linker |
Use minimal amount of cross-linking agent to achieve adequate fixation |
| Excessive tissue size in relation to fixative volume |
Reduce tissue size. Increase volume of fixative | |
| Penetration time of preservative solution |
Reduce tissue size. Use preservative with permeabilization reagents |
|
| Elevated storage temperature | Store tissue at appropriate temperature for preservation solution. Reduce storage temperature |
|
| Tissue hydration state | Low ambient humidity. Open specimen container |
Transport tissue in a closed container |
| Delay in transport/preservation | ||
| Post-analytical | ||
| Time delay to analysis | Lack of proper equipment, reagents, storage conditions |
Prepare reagents in advance. Plan procedure prior to retrieving samples |
| Malfunctioning equipment | Develop a plan to use an alternate source of equipment | |
| Poor/variable quality protein and/or nucleic acids results |
Delay in stabilizing tissue sample | Transport/preserve/fix tissue as soon as possible post excision |
| Elevated ambient temperature during tissue transport/processing |
Place samples on wet ice or in chilled container | |
| Inadequate fixation/preservation | Follow directions for type of fixation/tissue | |
| Use of post-mortem tissue samples | Limit ischemic conditions. Procure samples as soon as possible post-mortem |
|
| Differences in sample handling and processing |
Stabilize/preserve tissue as soon as possible post excision (time <20 min) |
|
| Obtain highly pure cell populations (>75%) | ||
| Freeze tissue in such a method as to ensure rapid, uniform cooling (<5 min). | ||
| Use RNAse-free precautions: wear gloves, use nucleic acid free plastic ware, clean work area with RNAse decontamination solutions | ||
| Add protease inhibitors to appropriate reagents | ||
| Extensive cross-linking due to fixation | Determine type of fixation, volume or size of tissue sample, depth of tissue within the tissue block |
|
| Inadequate removal of paraffin from formalin-fixed paraffin embedded tissue |
De-paraffinize in two changes of xylene for 5–15 min each | |