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REF add some notes to myself

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Nathan Dwarshuis 2021-07-27 12:26:45 -04:00
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tex/thesis.tex
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@ -698,6 +698,7 @@ Therefore, the proposed microcarrier system should enable greater expansion and
better retention of memory phenotype compared to current bead-based methods. better retention of memory phenotype compared to current bead-based methods.
\section{methods} \section{methods}
\subsection{dms functionalization} \subsection{dms functionalization}
\begin{figure*}[ht!] \begin{figure*}[ht!]
@ -834,6 +835,8 @@ Cells on the \glspl{dms} were visualized by adding \SI{0.5}{\ul}
\product{\acd{45}-\gls{af647}}{\bl}{368538}, incubating for \SI{1}{\hour}, and \product{\acd{45}-\gls{af647}}{\bl}{368538}, incubating for \SI{1}{\hour}, and
imaging on a spinning disk confocal microscope. imaging on a spinning disk confocal microscope.
% METHOD mtt staining and interior quantification
\subsection{quantification of apoptosis using Annexin-V} \subsection{quantification of apoptosis using Annexin-V}
Apoptosis was quantified using \gls{anv} according to the manufacturer's Apoptosis was quantified using \gls{anv} according to the manufacturer's
@ -905,6 +908,7 @@ Briefly, cells were washed once and stained with \product{biotinylated
BD Accuri. Readout was percent \gls{pe}+ cells as compared to secondary controls BD Accuri. Readout was percent \gls{pe}+ cells as compared to secondary controls
(\gls{pe}-\gls{stp} with no \gls{ptnl}). (\gls{pe}-\gls{stp} with no \gls{ptnl}).
% TODO add BCMA-CAR stuff
\subsection{car plasmid and lentiviral transduction} \subsection{car plasmid and lentiviral transduction}
The anti-CD19-CD8-CD137-CD3z \gls{car} with the EF1$\upalpha$ The anti-CD19-CD8-CD137-CD3z \gls{car} with the EF1$\upalpha$
@ -924,8 +928,6 @@ plates and incubated for another \SI{24}{\hour}. Cells and beads/\glspl{dms}
were removed from the retronectin plates using vigorous pipetting and were removed from the retronectin plates using vigorous pipetting and
transferred to another 96 well plate wherein expansion continued. transferred to another 96 well plate wherein expansion continued.
\subsection{statistical analysis} \subsection{statistical analysis}
For 1-way \gls{anova} analysis with Tukey multiple comparisons test, For 1-way \gls{anova} analysis with Tukey multiple comparisons test,
@ -947,7 +949,8 @@ lack-of-fit tests where replicates were present (to assess model fit in the
context of pure error). Statistical significance was evaluated at $\upalpha$ = context of pure error). Statistical significance was evaluated at $\upalpha$ =
0.05. 0.05.
% TODO add meta-analysis section % METHOD add meta-analysis
% METHOD add Grex
\section{results} \section{results}
@ -976,9 +979,8 @@ noted that the maximal \gls{mab} binding capacity occurred near \SI{50}{\nmol}
biotin input (which corresponded to \SI{2.5}{\nmol\per\mg\of{\dms}}) thus we biotin input (which corresponded to \SI{2.5}{\nmol\per\mg\of{\dms}}) thus we
used this in subsequent processes. used this in subsequent processes.
% TODO add paragraph explaining the qc stuff % RESULT add paragraph explaining the qc stuff
% RESULT add paragraph explaining the reaction kinetics stuff
% TODO add paragraph explaining the reaction kinetics stuff
% TODO flip the rows of this figure (right now the text is backward) % TODO flip the rows of this figure (right now the text is backward)
\begin{figure*}[ht!] \begin{figure*}[ht!]
@ -1135,7 +1137,6 @@ cells after \SI{14}{\day} were on the interior surface of the \glspl{dms}
\label{fig:dms_flowchart} \label{fig:dms_flowchart}
\end{figure*} \end{figure*}
% TODO add this to the methods section
% TODO double check the timing of this experiment (it might not be day 14) % TODO double check the timing of this experiment (it might not be day 14)
% TODO provide the regression results and coefficients from this % TODO provide the regression results and coefficients from this
\begin{figure*}[ht!] \begin{figure*}[ht!]
@ -1290,9 +1291,17 @@ showing that migration was likely independent of \gls{car} transduction.
\subcap{fig:car_production_migration}{Endpoint plot for transmigration assay \subcap{fig:car_production_migration}{Endpoint plot for transmigration assay
with \gls{anova}.} All data is from T cells expanded for \SI{14}{\day}. with \gls{anova}.} All data is from T cells expanded for \SI{14}{\day}.
} }
\label{fig:dms_phenotype} \label{fig:car_production}
\end{figure*} \end{figure*}
% FIGURE bcma results
\subsection{DMSs efficiently expand T cells in Grex bioreactors}
% FIGURE grex
% FIGURE luminex
% FIGURE grex + car
\subsection{DMSs do not leave antibodies attached to cell product} \subsection{DMSs do not leave antibodies attached to cell product}
We asked if \glspl{mab} from the \glspl{dms} detached from the \gls{dms} surface We asked if \glspl{mab} from the \glspl{dms} detached from the \gls{dms} surface
@ -1625,6 +1634,8 @@ provide these benefits.
\subsection{DOE shows optimal conditions for expanded potent T cells} \subsection{DOE shows optimal conditions for expanded potent T cells}
% TABLE luminex panel used
% TODO this plots proportions look dumb % TODO this plots proportions look dumb
\begin{figure*}[ht!] \begin{figure*}[ht!]
\begingroup \begingroup
@ -1699,7 +1710,7 @@ provide these benefits.
\label{fig:doe_responses} \label{fig:doe_responses}
\end{figure*} \end{figure*}
% TODO add DOE regression tables % TABLE DOE regression results
% TODO this section header sucks % TODO this section header sucks
\subsection{AI modeling reveals highly predictive species} \subsection{AI modeling reveals highly predictive species}