Design and Fabrication of Sustained Bacterial Release Scaffolds to Support the Microbiome

Author:

Klein Anne Marie1,Qosim Nanang123ORCID,Williams Gareth3ORCID,Edirisinghe Mohan1,Matharu Rupy Kaur4ORCID

Affiliation:

1. Department of Mechanical Engineering, University College London, Torrington Place, London WC1E 7JE, UK

2. Department of Mechanical Engineering, Politeknik Negeri Malang, Jl. Soekarno Hatta No. 9, Malang 65141, Jawa Timur, Indonesia

3. UCL School of Pharmacy, University College London, 29–39 Brunswick Square, London WC1N 1AX, UK

4. Department of Civil, Environmental & Geomatic Engineering, University College London, Chadwick Building, Gower Street, London WC1E 6BT, UK

Abstract

Fibres in the micro- and nanometre scale are suited to a broad range of applications, including drug delivery and tissue engineering. Electrospinning is the manufacturing method of choice, but it has some limitations. Novel pressure-driven fibre-forming techniques, like pressurised gyration (PG), overcome these limitations; however, the compatibility of PG with biological materials has not yet been evaluated in detail. For the first time, this limitation of PG was investigated by optimising PG for microbial cell processing and incorporating bacterial cultures into fibrous polymeric scaffolds for sustained release. Multiple polymer–solvent systems were trialled, including polyvinylpyrrolidone (PVP)/phosphate-buffered saline (PBS) 25% w/v, polyethylene oxide (PEO)/PBS 20% w/v, and PVP/ethanol 20% w/v. Rheological studies revealed the surface tension of the PVP/PBS, PEO/PBS, and PVP/ethanol polymer–solvent systems to be 73.2, 73.9, and 22.6 mN/m, respectively. Scanning electron microscopy showed the median fibre diameters to be between 9.8 μm and 26.1 μm, with PVP producing larger fibres. Overnight Bacillus subtilis cultures were then incorporated into the chosen polymeric solutions and processed into fibres using PG. The produced cell-loaded fibres were incubated in LB broth to assess the cell viability of the encapsulated cells. Colony counts post-incubation showed the PVP/PBS 25% fibres resulted in 60% bacterial growth, and PEO/PBS 20% fibres led to 47% bacterial growth, whereas PVP/ethanol 20% fibres did not lead to any bacterial growth. Based on the results gathered during this study, it can be concluded that PG offers a promising way of encapsulating cells and other sensitive biological products while having many notable advantages compared to electrospinning. This research demonstrates proof of concept research-based evidence and showcases the potential of pressurised gyration as a key disruptive innovation in probiotic delivery system design and manufacturing.

Funder

Lembaga Pengelola Dana Pendidikan (LPDP), The Ministry of Finance, The Republic of Indonesia

EPSRC

Publisher

MDPI AG

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