Membrane fatty acid heterogeneity of leukocyte classes is altered during in vitro cultivation but can be restored with ad-hoc lipid supplementation

Paola Poggi; Roberto Mirabella; Simona Neri; Elisa Assirelli; Paolo Dolzani; Erminia Mariani; Philip C Calder; Alexandros Chatgilialoglu

doi:10.1186/s12944-015-0166-3

Membrane fatty acid heterogeneity of leukocyte classes is altered during in vitro cultivation but can be restored with ad-hoc lipid supplementation

Lipids Health Dis. 2015 Dec 24:14:165. doi: 10.1186/s12944-015-0166-3.

Authors

Paola Poggi¹, Roberto Mirabella², Simona Neri³, Elisa Assirelli⁴, Paolo Dolzani⁵, Erminia Mariani^{6

7}, Philip C Calder^{8

9

10}, Alexandros Chatgilialoglu¹¹

Affiliations

¹ Remembrane Srl, via Selice 84/A, 40026, Imola, Italy. paola.poggi@remembrane.com.
² Remembrane Srl, via Selice 84/A, 40026, Imola, Italy. roberto.mirabella@remembrane.com.
³ Laboratory of Immunorheumatology and Tissue Regeneration/RAMSES, Rizzoli Orthopedic Institute, via di Barbiano 1/10, 40136, Bologna, Italy. simona.neri@ior.it.
⁴ Laboratory of Immunorheumatology and Tissue Regeneration/RAMSES, Rizzoli Orthopedic Institute, via di Barbiano 1/10, 40136, Bologna, Italy. elisa.assirelli@ior.it.
⁵ Laboratory of Immunorheumatology and Tissue Regeneration/RAMSES, Rizzoli Orthopedic Institute, via di Barbiano 1/10, 40136, Bologna, Italy. paolo.dolzani@ior.it.
⁶ Laboratory of Immunorheumatology and Tissue Regeneration/RAMSES, Rizzoli Orthopedic Institute, via di Barbiano 1/10, 40136, Bologna, Italy. erminia.mariani@unibo.it.
⁷ Department of Medical and Surgical Sciences, University of Bologna, Bologna, Italy. erminia.mariani@unibo.it.
⁸ Human Development and Health Academic Unit, Faculty of Medicine, University of Southampton, Tremona Road, SO16 6YD, Southampton, UK. p.c.calder@soton.ac.uk.
⁹ NIHR Southampton Biomedical Research Centre, University Hospital Southampton NHS Foundation Trust and University of Southampton, Southampton, UK. p.c.calder@soton.ac.uk.
¹⁰ Department of Biological Sciences, Faculty of Science, King Abdulaziz University, Jeddah, Saudi Arabia. p.c.calder@soton.ac.uk.
¹¹ Remembrane Srl, via Selice 84/A, 40026, Imola, Italy. alex.chatgilialoglu@remembrane.com.

Abstract

Background: The cell membrane is a primary and fundamental player in most cellular processes, and fatty acids form a major structural component of cell membranes. The aim of this study was to compare the membrane fatty acid profiles of different human blood leukocytes and selected cell lines, to identify the effects of in vitro culture on fatty acid profiles, and to test medium supplements for their effect on fatty acid profiles.

Methods: Different classes of leukocytes were isolated from human blood and their membrane fatty acid profiles were analysed and compared. After culturing in vitro immortalised and primary leukocytes, membrane fatty acids were analysed and compared. Finally, different lipid formulations were developed and used for supplementing leukocytes in vitro in an effort to maintain the in vivo fatty acid profile. Descriptive and analytical tests were performed to compare the obtained fatty acid profiles.

Results: Membrane fatty acid profiles of primary human CD4(+) T-lymphocytes, CD8(+) T-lymphocytes, B-lymphocytes and monocytes differed. Moreover, there were differences among Jurkat, Raji and THP-1 cell lines and the corresponding primary leukocyte classes, as well as between freshly prepared and in vitro cultured primary lymphocytes. A lipid supplement was able to maintain cultured Jurkat cells with a membrane fatty acid profile almost identical to that of the primary CD4(+) T-lymphocytes. Finally, variations in the lipid supplement composition enabled the development of Jurkat cells with different membrane fatty acid profiles characterising different physiological or pathological human conditions.

Conclusions: Each leukocyte class has its own specific membrane fatty acid profile in vivo. Cultured primary leukocytes and immortalized leukocytic cells display different membrane fatty acid profiles when compared to their respective in vivo counterparts. The membrane fatty acid composition of cultured cells can be restored to reflect that of the corresponding in vivo condition through use of optimised lipid supplementation. Typical physiological or pathological leukocyte membrane fatty acid profiles can be obtained by tuning in vitro fatty acid supplementation.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

B-Lymphocytes / chemistry*
B-Lymphocytes / drug effects
B-Lymphocytes / metabolism
CD4-Positive T-Lymphocytes / chemistry*
CD4-Positive T-Lymphocytes / drug effects
CD4-Positive T-Lymphocytes / metabolism
CD8-Positive T-Lymphocytes / chemistry*
CD8-Positive T-Lymphocytes / drug effects
CD8-Positive T-Lymphocytes / metabolism
Cell Membrane / chemistry
Cell Membrane / drug effects
Chromatography, Gas
Culture Media / chemistry
Culture Media / pharmacology
Fatty Acids / isolation & purification*
Fatty Acids / metabolism
Humans
Jurkat Cells
Membrane Fluidity / drug effects
Membrane Lipids / isolation & purification*
Membrane Lipids / metabolism
Monocytes / chemistry*
Monocytes / drug effects
Monocytes / metabolism
Primary Cell Culture

Substances

Culture Media
Fatty Acids
Membrane Lipids