TY  - GEN
A1  - Moradian, Hanieh
A1  - Roch, Toralf
A1  - Lendlein, Andreas
A1  - Gossen, Manfred
T1  - mRNA transfection-induced activation of primary human monocytes and macrophages
BT  - Dependence on carrier system and nucleotide modifcation
T2  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe
N2  - Monocytes and macrophages are key players in maintaining immune homeostasis. Identifying strategies to manipulate their functions via gene delivery is thus of great interest for immunological research and biomedical applications. We set out to establish conditions for mRNA transfection in hard-to-transfect primary human monocytes and monocyte-derived macrophages due to the great potential of gene expression from in vitro transcribed mRNA for modulating cell phenotypes. mRNA doses, nucleotide modifications, and different carriers were systematically explored in order to optimize high mRNA transfer rates while minimizing cell stress and immune activation. We selected three commercially available mRNA transfection reagents including liposome and polymer-based formulations, covering different application spectra. Our results demonstrate that liposomal reagents can particularly combine high gene transfer rates with only moderate immune cell activation. For the latter, use of specific nucleotide modifications proved essential. In addition to improving efficacy of gene transfer, our findings address discrete aspects of innate immune activation using cytokine and surface marker expression, as well as cell viability as key readouts to judge overall transfection efficiency. The impact of this study goes beyond optimizing transfection conditions for immune cells, by providing a framework for assessing new gene carrier systems for monocyte and macrophage, tailored to specific applications.
T3  - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 1403 
KW  - sirna transfection
KW  - mediated delivery
KW  - gene delivery
KW  - efficient
KW  - immunogenicity
KW  - lipoplexes
KW  - cells
KW  - therapeutics
KW  - polarization
KW  - pathways
Y1  - 2020
U6  - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-515694
SN  - 1866-8372
IS  - 1
ER  - 
TY  - JOUR
A1  - Moradian, Hanieh
A1  - Roch, Toralf
A1  - Lendlein, Andreas
A1  - Gossen, Manfred
T1  - mRNA transfection-induced activation of primary human monocytes and macrophages
BT  - Dependence on carrier system and nucleotide modifcation
JF  - Scientific reports
N2  - Monocytes and macrophages are key players in maintaining immune homeostasis. Identifying strategies to manipulate their functions via gene delivery is thus of great interest for immunological research and biomedical applications. We set out to establish conditions for mRNA transfection in hard-to-transfect primary human monocytes and monocyte-derived macrophages due to the great potential of gene expression from in vitro transcribed mRNA for modulating cell phenotypes. mRNA doses, nucleotide modifications, and different carriers were systematically explored in order to optimize high mRNA transfer rates while minimizing cell stress and immune activation. We selected three commercially available mRNA transfection reagents including liposome and polymer-based formulations, covering different application spectra. Our results demonstrate that liposomal reagents can particularly combine high gene transfer rates with only moderate immune cell activation. For the latter, use of specific nucleotide modifications proved essential. In addition to improving efficacy of gene transfer, our findings address discrete aspects of innate immune activation using cytokine and surface marker expression, as well as cell viability as key readouts to judge overall transfection efficiency. The impact of this study goes beyond optimizing transfection conditions for immune cells, by providing a framework for assessing new gene carrier systems for monocyte and macrophage, tailored to specific applications.
KW  - sirna transfection
KW  - mediated delivery
KW  - gene delivery
KW  - efficient
KW  - immunogenicity
KW  - lipoplexes
KW  - cells
KW  - therapeutics
KW  - polarization
KW  - pathways
Y1  - 2020
U6  - https://doi.org/10.1038/s41598-020-60506-4
SN  - 2045-2322
VL  - 10
IS  - 1
SP  - 1
EP  - 15
PB  - Springer Nature
CY  - London
ER  - 
TY  - JOUR
A1  - Bhuvanesh, Thanga
A1  - Saretia, Shivam
A1  - Roch, Toralf
A1  - Schöne, Anne-Christin
A1  - Rottke, Falko O.
A1  - Kratz, Karl
A1  - Wang, Weiwei
A1  - Ma, Nan
A1  - Schulz, Burkhard
A1  - Lendlein, Andreas
T1  - Langmuir-Schaefer films of fibronectin as designed biointerfaces for culturing stem cells
JF  - Polymers for advanced technologies
N2  - Glycoproteins adsorbing on an implant upon contact with body fluids can affect the biological response in vitro and in vivo, depending on the type and conformation of the adsorbed biomacromolecules. However, this process is poorly characterized and so far not controllable. Here, protein monolayers of high molecular cohesion with defined density are transferred onto polymeric substrates by the Langmuir-Schaefer (LS) technique and were compared with solution deposition (SO) method. It is hypothesized that on polydimethylsiloxane (PDMS), a substrate with poor cell adhesion capacity, the fibronectin (FN) layers generated by the LS and SO methods will differ in their organization, subsequently facilitating differential stem cell adhesion behavior. Indeed, atomic force microscopy visualization and immunofluorescence images indicated that organization of the FN layer immobilized on PDMS was uniform and homogeneous. In contrast, FN deposited by SO method was rather heterogeneous with appearance of structures resembling protein aggregates. Human mesenchymal stem cells showed reduced absolute numbers of adherent cells, and the vinculin expression seemed to be higher and more homogenously distributed after seeding on PDMS equipped with FN by LS in comparison with PDMS equipped with FN by SO. These divergent responses could be attributed to differences in the availability of adhesion molecule ligands such as the Arg-Gly-Asp (RGD) peptide sequence presented at the interface. The LS method allows to control the protein layer characteristics, including the thickness and the protein orientation or conformation, which can be harnessed to direct stem cell responses to defined outcomes, including migration and differentiation. Copyright (c) 2016 John Wiley & Sons, Ltd.
KW  - Langmuir-Schaefer method
KW  - protein adsorption
KW  - stem cell adhesion
KW  - cell culture
KW  - fibronectin
Y1  - 2017
U6  - https://doi.org/10.1002/pat.3910
SN  - 1042-7147
SN  - 1099-1581
VL  - 28
SP  - 1305
EP  - 1311
PB  - Wiley
CY  - Hoboken
ER  - 
TY  - JOUR
A1  - Bhaskar, Thanga Bhuvanesh Vijaya
A1  - Ma, Nan
A1  - Lendlein, Andreas
A1  - Roch, Toralf
T1  - The interaction of human macrophage subsets with silicone as a biomaterial
JF  - Clinical hemorheology and microcirculation : blood flow and vessels
N2  - Silicones are widely used as biomaterials for medical devices such as extracorporeal equipments. However, there is often conflicting evidence about their supposed cell-and histocompatibility. Macrophages could mediate silicone-induced adverse responses such as foreign body reaction and fibrous encapsulation. The polarization behaviour of macrophages could determine the clinical outcome after implantation of biomaterials. Induction of classically activated macrophages (CAM) may induce and support uncontrolled inflammatory responses and undesired material degradation. In contrast, polarization into alternatively activated macrophages (AAM) is assumed to support healing processes and implant integration.
 This study compared the interaction of non-polarized macrophages (M0), CAM, and AAM with commercially available tissue culture polystyrene (TCP) and a medical grade silicone-based biomaterial, regarding the secretion of inflammatory mediators such as cytokines and chemokines. Firstly, by using the Limulus amoebocyte lysate (LAL) test the silicone films were shown to be free of soluble endotoxins, which is the prerequisite to investigate their interaction with primary immune cells. Primary human monocyte-derived macrophages (M0) were polarized into CAM and AAM by addition of suitable differentiation factors. These macrophage subsets were incubated on the materials for 24 hours and their viability and cytokine secretion was assessed. In comparison to TCP, cell adhesion was lower on silicone after 24 hours for all three macrophage subsets. However, compared to TCP, silicone induced higher levels of certain inflammatory and chemotactic cytokines in M0, CAM, and AAM macrophage subsets.
 Conclusively, it was shown that silicone has the ability to induce a pro-inflammatory state to different magnitudes dependent on the macrophage subsets. This priming of the macrophage phenotype by silicone could explain the incidence of severe foreign body complications observed in vivo.
KW  - Biomaterials
KW  - silicone
KW  - macrophage subsets
KW  - cytokines/chemokines
Y1  - 2015
U6  - https://doi.org/10.3233/CH-151991
SN  - 1386-0291
SN  - 1875-8622
VL  - 61
IS  - 2
SP  - 119
EP  - 133
PB  - IOS Press
CY  - Amsterdam
ER  -