A practical approach for the validation of sterility, endotoxin and potency testing of bone marrow mononucleated cells used in cardiac regeneration in compliance with good manufacturing practice

Sabrina Soncin; Viviana Lo Cicero; Giuseppe Astori; Gianni Soldati; Mauro Gola; Daniel Sürder; Tiziano Moccetti

doi:10.1186/1479-5876-7-78

A practical approach for the validation of sterility, endotoxin and potency testing of bone marrow mononucleated cells used in cardiac regeneration in compliance with good manufacturing practice

J Transl Med. 2009 Sep 8:7:78. doi: 10.1186/1479-5876-7-78.

Authors

Sabrina Soncin¹, Viviana Lo Cicero, Giuseppe Astori, Gianni Soldati, Mauro Gola, Daniel Sürder, Tiziano Moccetti

Affiliation

¹ The Cell Therapy Unit, Cardiocentro Ticino, Via Tesserete 48, CH-6900 Lugano, Switzerland. sabrina.soncin@cardiocentro.org

Abstract

Background: Main scope of the EU and FDA regulations is to establish a classification criterion for advanced therapy medicinal products (ATMP). Regulations require that ATMPs must be prepared under good manufacturing practice (GMP). We have validated a commercial system for the determination of bacterial endotoxins in compliance with EU Pharmacopoeia 2.6.14, the sterility testing in compliance with EU Pharmacopoeia 2.6.1 and a potency assay in an ATMP constituted of mononucleated cells used in cardiac regeneration.

Methods: For the potency assay, cells were placed in the upper part of a modified Boyden chamber containing Endocult Basal Medium with supplements and transmigrated cells were scored. The invasion index was expressed as the ratio between the numbers of invading cells relative to cell migration through a control insert membrane. For endotoxins, we used a commercially available system based on the kinetic chromogenic LAL-test. Validation of sterility was performed by direct inoculation of TSB and FTM media with the cell product following Eu Ph 2.6.1 guideline.

Results and discussion: The calculated MVD and endotoxin limit were 780x and 39 EU/ml respectively. The 1:10 and 1:100 dilutions were selected for the validation. For sterility, all the FTM cultures were positive after 3 days. For TSB cultures, Mycetes and B. subtilis were positive after 5 and 3 days respectively. The detection limit was 1-10 colonies. A total of four invasion assay were performed: the calculated invasion index was 28.89 +/- 16.82% (mean +/- SD).

Conclusion: We have validated a strategy for endotoxin, sterility and potency testing in an ATMP used in cardiac regeneration. Unlike pharmaceutical products, many stem-cell-based products may originate in hospitals where personnel are unfamiliar with the applicable regulations. As new ATMPs are developed, the regulatory framework is likely to evolve. Meanwhile, existing regulations provide an appropriate structure for ensuring the safety and efficacy of the next generation of ATMPs. Personnel must be adequately trained on relevant methods and their application to stem-cell-based products.

MeSH terms

Biological Assay / methods
Bone Marrow Cells / cytology
Bone Marrow Cells / physiology*
Cell Movement / physiology
Endotoxins / metabolism*
European Union
Heart / physiology*
Humans
Leukocytes, Mononuclear / cytology
Leukocytes, Mononuclear / physiology*
Manufactured Materials* / microbiology
Manufactured Materials* / standards
Myocardium / cytology*
Pharmacopoeias as Topic / standards
Regeneration / physiology*
Reproducibility of Results
Sterilization / methods
Sterilization / standards
United States

Substances

Endotoxins