ADD reaction kinetics results paragraphs
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@ -96,6 +96,7 @@
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\newacronym{tmb}{TMB}{3,3',5,5'-Tetramethylbenzidine}
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\newacronym{tmb}{TMB}{3,3',5,5'-Tetramethylbenzidine}
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\newacronym{gvhd}{GVHD}{graft-vs-host disease}
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\newacronym{gvhd}{GVHD}{graft-vs-host disease}
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\newacronym{bcma}{BCMA}{B-cell maturation antigen}
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\newacronym{bcma}{BCMA}{B-cell maturation antigen}
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\newacronym{di}{DI}{deionized}
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%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%
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%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%
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% SI units for uber nerds
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% SI units for uber nerds
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@ -951,6 +952,8 @@ transferred to another 96 well plate wherein expansion continued.
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% METHOD snb decay curve generation and analysis (including the equation used to
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% METHOD snb decay curve generation and analysis (including the equation used to
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% fit the data)
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% fit the data)
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% METHOD add reaction kinetics diffusion mathy stuff
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\subsection{Luminex Analysis}
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\subsection{Luminex Analysis}
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Luminex was performed using a \product{ProcartaPlex kit}{\thermo}{custom} for
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Luminex was performed using a \product{ProcartaPlex kit}{\thermo}{custom} for
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@ -1148,7 +1151,38 @@ higher, further showing that the decay of \gls{snb} is not a concern.
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\label{fig:dms_flowchart}
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\label{fig:dms_flowchart}
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\end{figure*}
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\end{figure*}
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% RESULT add paragraph explaining the reaction kinetics stuff
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We also investigated the reaction kinetics of all three coating steps.
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To quantify the reaction kinetics of the biotin binding step, we reacted
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multiple batches of microcarriers at \gls{rt} with
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\gls{20}{\mg\of{\carrier}\per\ml} with \gls{snb} in parallel and sacrificially
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analyzed each at varying timepoints using the \gls{haba} assay. This was
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performed at two different concentrations. We observed that for either
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concentration, the reaction was over in \SIrange{20}{30}{\minute}
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(\cref{fig:dms_biotin_rxn_mass}). Furthermore, when put in terms of fraction of
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input \gls{snb}, we observed that the curves are almost identical
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(\cref{fig:dms_biotin_rxn_frac}). Given this, the reaction step for biotin
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attached was set to \gls{30}{\minute}.
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% TODO these numbers might be totally incorrect
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Next, we quantified the amount of \gls{stp} reacted with the surface of the
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biotin-coated microcarriers. Different batches of biotin-coated \glspl{dms} were
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coated with \SI{40}{\ug\per\ml} \gls{stp} and sampled at various timepoints
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using the \gls{bca} assay to indirectly quantify the amount of attached
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\gls{stp} mass. We found this reaction took \SI{45}{\minute}
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(\cref{fig:dms_stp_per_time}).
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% TODO find real numbers for this
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Finally, we used the reaction data from the \gls{stp} binding curve to estimate
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the \gls{mab} binding curve. Assuming a quasi-steady-state paradigm, we
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estimated that the diffusion rate coefficient for the microcarriers was
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{\#}{diffusion rate}. Using this diffusion rate and the maximum mass of
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\glspl{mab} bound the microcarriers (\cref{fig:mab_coating}), we estimated that
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the \gls{mab} reaction should proceed in {\#}{mab curve}.
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% TODO add additional paragraph about how this diffusion coefficient was used to
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% estimate the wash step times.
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\begin{figure*}[ht!]
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\begin{figure*}[ht!]
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\begingroup
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\begingroup
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