ADD a bunch of background on microcarriers

2021-08-01 18:42:53 -04:00 · 2021-08-01 18:42:53 -04:00 · 8f7ee97f0a
parent bead38f3cd
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@ -569,6 +569,68 @@ present our final conclusions in Chapter~\ref{conclusions}.
 % TODO consider adding a separate section on microcarriers and their use in
 % bioprocess
 % TODO add stuff about T cell licensing
 \subsection{microcarriers in bioprocessing}
 % https://www.sciencedirect.com/science/article/pii/S0928493118338001#bb0010
 Microcarriers have historically been used to grow a number of adherent cell
 types for a variety of applications. They were introduced in 1967 as a means to
 grow adherent cells `in suspension', effectively turning a 2D flask system into
 a 3D culture system (https://www.nature.com/articles/216064a0.pdf).
 Microcarriers are generally spherical and are several hundred \si{\um} in
 diameter, which means they collectively have a much higher surface area than a
 traditional flask when matched for volume. Consequently, this means that
 microcarrier-based cultures can operate with much lower footprints than
 flask-like systems. Microcarriers also allow cell culture to operate more like a
 traditional chemical engineering process, wherein a stirred tank bioreactor may
 be employed to enhance oxygen transfer, maintain pH, and continuously supply
 nutrients ().
 A variety of microcarriers have been designed, primarily differing in their
 choice of material and macroporous structure. Key concerns have been cell
 attachment at the beginning of culture and cell detachment at the harvesting
 step; these have largely driven the nature of the material and structures
 employed. Many microcarriers simply use polystyrene (the material used for
 tissue culture flasks and dishes in general) with no modification (SoloHill
 Plastic, Nunc Biosilon), with a cationic surface charge (SoloHill Hillex) or
 coated with an \gls{ecm} protein such as collagen (SoloHill Fact III). Other
 base materials have been used such as dextran (GE Healthcare Cytodex), cellulose
 (GE Healthcare Cytopore), and glass (Sigma Aldrich G2767), all with none or
 similar surface modifications. Additionally, some microcarriers such as
 \gls{cus} and \gls{cug} are composed entirely out of protein (in these cases,
 porcine collagen) which also allows the microcarriers to be enzymatically
 degraded. In the case of non-protein materials, cells may still be detached
 using enzymes but these require similar methods to those currently used in
 flasks such as trypsin which target the cellular \gls{ecm} directly. Since
 trypsin and related enzymes tends to be harsh on cells, an advantage of using
 entirely protein-based microcarriers is that they can be degraded using a much
 safer enzyme such as collagenase, at the cost of being more expensive and also
 being harder to make \gls{gmp}-compliant. Going one step further, some
 microcarriers are composed of a naturally degrading scaffold such as alginate,
 which do not need an enzyme for degradation but are limited in that the
 degradation process is less controllable. Finally, microcarriers can differ in
 their overall structure. \gls{cug} and \gls{cus} microcarriers as well as the
 Cytopore microcarriers are macroporous, meaning they have a porous network in
 which cells can attach throughout their interior. This drastically increases the
 effective surface area and consequently the number of cells which may be grown
 per unit volume. Other microcarriers are microporous (eg only to small
 molecules) or not porous at all (eg polystyrene) in which case the cells can
 only grow on the surface.
 % https://www.sciencedirect.com/science/article/pii/S0734975013000657
 % https://link.springer.com/article/10.1023/A:1008038609967
 % https://onlinelibrary.wiley.com/doi/full/10.1002/bit.23289
 Microcarriers have seen the most use in growing \gls{cho} cells and hybridomas
 in the case of protein manufacturing (eg \gls{igg} production) as well as
 pluripotent stem cells and mesenchymal stromal cells more recently in the case
 of cell manufacturing\cite{Heathman2015, Sart2011}. Interestingly, some groups
 have even explored using biodegradable microcarriers \invivo{} as a delivery
 vehicle for stem cell therapies in the context of regenerative medicine.
 However, the characteristic shared by all the cell types in this application is
 the fact that they are adherent. In this work, we explore the use of
 microcarrier for T cells, which are naturally non-adherent.
 \subsection*{current T cell manufacturing technologies}
 \Gls{car} T cell therapy has received great interest from both academia and
@ -621,20 +683,6 @@ cytokine release properties and ability to resist exhaustion\cite{Wang2018,
  Yang2017}, and no method exists to preferentially expand the CD4 population
 compared to state-of-the-art systems.
 Here we propose a method using microcarriers functionalized with \acd{3} and
 \acd{28} \glspl{mab} for use in T cell expansion cultures. Microcarriers have
 historically been used throughout the bioprocess industry for adherent cultures
 such as stem cells and \gls{cho} cells, but not with suspension cells such as T
 cells\cite{Heathman2015, Sart2011}. The carriers have a macroporous structure
 that allows T cells to grow inside and along the surface, providing ample
 cell-cell contact for enhanced autocrine and paracrine signaling. Furthermore,
 the carriers are composed of gelatin, which is a collagen derivative and
 therefore has adhesion domains that are also present within the lymph nodes.
 Finally, the 3D surface of the carriers provides a larger contact area for T
 cells to interact with the \glspl{mab} relative to beads; this may better
 emulate the large contact surface area that occurs between T cells and
 \glspl{dc}.
 \subsection*{integrins and T cell signaling}
 Because the microcarriers used in this work are derived from collagen, one key