Growth Protocol:	Before development, cells were grown in HL5 (Formedium, UK).
Treatment Protocol:	Cells were developed for 14 h on Whatman #50 filter paper in a humified chamber. Developed cells were disaggregated in KK2 + 20 mM EDTA then dedifferentiated in HL5 growth medium as a shaken suspension. Start times of development and dedifferentiation were staggered to allow simultaneous collection of samples into ice-cold KK2 at 0, 1, 2, 3, 4, 5 and 6 h of dedifferentiation.
Extract Protocol:	Cell suspensions from different timepoints were pooled before loading onto the 10X Chromium Single Cell A Chip using the Chromium 3' Library and Gel Bead Kit v2. Samples were split between two chip inlets and treated as technical replicates
Library Construction Protocol:	The purified GEM-RT product was subjected to 14 cycles of cDNA amplification. 35 microlitres of cDNA was used to prepare the 10X 3' RNA library, with 12/11 cycles used for sample index PCR. Final libraries were run on a NextSeq500 mid-output 150-cycle kit with a 26[8]98 cycle configuration to generate 130 million read pairs in total.

Molecule Type:	poly(A)+ RNA
Library Source:
Library Layout:	PAIRED
Library Strand:	-
Platform:	ILLUMINA
Instrument Model:	NextSeq 500
Strand-Specific:	-

Data Resource	GEN Sample ID	GEN Dataset ID	Project ID	BioProject ID	Sample ID	Sample Name	BioSample ID	Sample Accession	Experiment Accession	Release Date	Submission Date	Update Date	Species	Race	Ethnicity	Age	Age Unit	Gender	Source Name	Tissue	Cell Type	Cell Subtype	Cell Line	Disease	Disease State	Development Stage	Mutation	Phenotype	Case Detail	Control Detail	Growth Protocol	Treatment Protocol	Extract Protocol	Library Construction Protocol	Molecule Type	Library Layout	Strand-Specific	Library Strand	Spike-In	Strategy	Platform	Instrument Model	Cell Number	Reads Number	Gbases	AvgSpotLen1	AvgSpotLen2	Uniq Mapping Rate	Multiple Mapping Rate	Coverage Rate