ADD methods to aim 2b
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@ -53,6 +53,8 @@
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\newacronym{pdms}{PDMS}{polydimethylsiloxane}
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\newacronym{dc}{DC}{dendritic cell}
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\newacronym{il2}{IL2}{interleukin 2}
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\newacronym{il15}{IL15}{interleukin 15}
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\newacronym{il15r}{IL15R}{interleukin 15 receptor}
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\newacronym{rhil2}{rhIL2}{recombinant human interleukin 2}
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\newacronym{apc}{APC}{antigen presenting cell}
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\newacronym{mhc}{MHC}{major histocompatibility complex}
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@ -104,7 +106,11 @@
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\newacronym{fcs}{FCS}{flow cytometry standard}
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\newacronym{ivis}{ivis}{in vivo imaging system}
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\newacronym{iacuc}{IACUC}{institutional animal care and use committee}
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\newacronym{hbss}{HBSS}{Hank's buffered saline solution}
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\newacronym{leaf}{LEAF}{low endotoxin, azide-free}
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\newacronym{cytof}{CyTOF}{cytometry time-of-flight}
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\newacronym{spade}{SPADE}{spanning-tree progression analysis of
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density-normalized events}
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%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%%
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% SI units for uber nerds
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@ -2076,6 +2082,64 @@ provide these benefits.
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\section{introduction}
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\section{methods}
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\subsection{collagenase digestion}
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% TODO The concentration for the surface marker cleavage experiment was much
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% higher, if that matters
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\glspl{dms} were digested in active T cell cultures via addition of sterile
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\product{\gls{colb}}{Sigma}{11088807001} or
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\product{\gls{cold}}{Sigma}{11088858001}. Collagenase was dissolved in
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\product{\gls{hbss}}{Gibco}{14025-076} or
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\product{TexMACS}{\miltenyi}{170-076-307} at approximately \SI{100}{\ug\per\ml}.
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This solution was added to T cell cultures at a 1:1 ratio in place of plain
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media normally used to feed the cells during the regular media addition cycle at
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day 4. Cultures were then incubated as described in \cref{sec:tcellculture}, and
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the \glspl{dms} were verified to have been digested after \SI{24}{\hour}.
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\subsection{mass cytometry and clustering analysis}
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T cells were stained using a \product{34 \gls{cytof} marker
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panel}{Fluidigm}{201322} and \product{cisplatin}{Fluidigm}{201064} which were
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used according to the manufacturer’s instructions. \numrange{2e6}{3e6} stained
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cells per group were analyzed on a Fluidigm Helios.
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% FIGURE add the spade gating diagram from the paper
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Unbiased cell clusters were obtained using \gls{spade} analysis by pooling three
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representative \gls{fcs} files and running the \gls{spade} pipeline with k-means
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clustering (k = 100), arcsinh transformation with cofactor 5, density
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calculation neighborhood size of 5 and local density approximation factor of
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1.5, target density of 20000 cells, and outlier density cutoff of
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\SI{1}{\percent}. All markers in the \gls{cytof} panel were used in the analysis
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\subsection{integrin blocking experiments}
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To block \gls{a2b1} and \gls{a2b2}, active T cell cultures with \gls{dms} were
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supplemented with \product{\anti{\gls{a2b1}}}{Sigma}{MAB1973Z} and
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\product{\anti{\gls{a2b2}}}{Sigma}{MAB1950Z} (both \gls{leaf}) at indicated
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concentrations and timepoints. T cells were grown as described in
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\cref{sec:tcellculture}.
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\gls{a2b1} and \gls{a2b2} were verified to be present on active T cell cultures
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by staining with \product{\anti{\gls{a2b1}}-\gls{apc}}{\bl}{328313} and
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\product{\anti{\gls{a2b2}}-\gls{fitc}}{\bl}{359305} on day 6 of culture and
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analyzing via a BD Accuri flow cytometer.
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\subsection{IL15 blocking experiments}
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To block the \gls{il15r}, we supplemented T cell
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cultures activated with \gls{dms} with either
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\product{\anti{\gls{il15r}}}{Rnd}{AF247} or \product{\gls{igg} isotype
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control}{RnD}{AB-108-C} at the indicated timepoints and concentrations. T
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cells were grown as otherwise described in \cref{sec:tcellculture} with the
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exception that volumes were split by $\frac{1}{3}$ to keep the culture volume
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constant and minimize the amount of \gls{mab} required.
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To block soluble \gls{il15}, we supplemented analogously with
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\product{\anti{\gls{il15}}}{RnD}{EEP0419081} or \product{\gls{igg} isotype
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control}{\bl}{B236633}.
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\section{results}
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\subsection{adding or removing DMSs alters expansion and phenotype}
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