Data from: Phagolysosomes break down the membrane of a non-apoptotic corpse independent of macroautophagy
Data files
Oct 04, 2024 version files 66.69 GB
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PLoS_One_Figure_Guide.csv
6.35 KB
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README.md
7.98 KB
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WEH683_Archive.zip
4.82 GB
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WEH684_Archive.zip
6.60 GB
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WEH696_Archive.zip
3.57 GB
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WEH700_Archive.zip
11.18 GB
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WEH708_Archive.zip
3.28 GB
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WEH714_Archive.zip
11.65 GB
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WEH722_Archive.zip
3.74 GB
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WEH728_Archive.zip
882.64 MB
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WEH729_Archive.zip
1.51 GB
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WEH731_Archive.zip
13.96 GB
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WEH734_Archive.zip
890.47 MB
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WEH739_Archive.zip
1.32 GB
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WEH755_Archive.zip
1.38 GB
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WEH95_Archive.zip
1.91 GB
Abstract
Cell corpses must be cleared in an efficient manner to maintain tissue homeostasis and regulate immune responses. Ubiquitin-like Atg8/LC3 family proteins promote the degradation of membranes and internal cargo during both macroautophagy and corpse clearance, raising the question how macroautophagy contributes to corpse clearance. Studying the clearance of non-apoptotic dying polar bodies in Caenorhabditis elegans embryos, we show that the LC3 ortholog LGG-2 is enriched inside the polar body phagolysosome independent of autophagosome formation. We demonstrate that ATG-16.1 and ATG-16.2, which promote membrane association of lipidated Atg8/LC3 proteins, redundantly promote polar body membrane breakdown in phagolysosomes independent of their role in macroautophagy. We also show that the lipid scramblase ATG-9 is needed for autophagosome formation in early embryos but is dispensable for timely polar body membrane breakdown or protein cargo degradation. These findings demonstrate that macroautophagy is not required to promote polar body degradation, in contrast to recent findings with apoptotic corpse clearance in C. elegans embryos. Determining how factors regulating Atg8/LC3 promote the breakdown of different types of cell corpses in distinct cell types or metabolic states is likely to give insights into the mechanisms of immunoregulation during normal development, physiology, and disease.
https://doi.org/10.5061/dryad.sj3tx96df
Description of the data and file structure
In the study by Kolli, Kline et al. entitled “Phagolysosomes break down the membrane of a non-apoptotic corpse independent of macroautophagy”, we confirm that ATG-9 and ATG-16.2 are required for normal autophagosome biogenesis in C. elegans early embryos. In the absence of autophagosomes, we find no delay in corpse membrane breakdown, no disruption in LGG-2 localization inside the polar body phagolysosome, and no delay in degradation of a corpse cargo protein. These data suggest that autophagosomes are not required for phagolysosome maturation in early embryos. We also find that ATG-16.1 and ATG-16.2 redundantly promote polar body membrane breakdown. In combination with the published role for the lipidation factor ATG-7 (Fazeli et al., Cell Rep 2016), these data suggest that the association of lipidated Atg8/LC3 with a non-autophagic membrane is important for the phagocytic clearance of a non-apoptotic corpse.
The imaging data in the archived .sld files are viewable for free in SlideBook Reader software or after installing the SlideBook Bio-Formats plugin in FIJI or ImageJ software (Linked below under Code/software).
Files and variables
File: PLoS One Figure Guide.csv
Description: Spreadsheet detailing where the raw imaging data in the figures of the Kolli, Kline et al. manuscript are found in the following zip archives containing sld files.
File: WEH95_Archive.zip
Description: Time-lapse imaging data of wild type control embryos with green membrane marker degraded in somatic cells and red histones
Genotype: xnIs390[pie-1::GFP::ZF1::PH(PLCdelta1), unc-119(+)]; unc-119(ed3) III; Is[mCherry::HistoneH2B] IV
Contains WEH95-10%.sld
File: WEH683_Archive.zip
Description: Time-lapse imaging data of atg-16.1 mutant embryos with green membrane degraded in somatic cells and red histones
Genotype: xnIs390[pie-1::GFP::ZF1::PH(PLC1delta1), unc-119(+)] II; Is[mCherry::HistoneH2B] IV; atg-16.1(gk668615[Q356Stop]) X
Contains WEH683-10%.sld and WEH683-10%_2.sld
File: WEH684_Archive.zip
Description: Time-lapse imaging data of atg-16.2 mutant embryos with green membrane degraded in somatic cells and red histones
Genotype: atg-16.2(ok3224) xnIs390[pie-1::GFP::ZF1::PH(PLC1delta1), unc-119(+)] II; Is[mCherry::HistoneH2B] IV
Contains WEH684-10%.sld, WEH684-10%_2.sld, WEH684-10%_3.sld, WEH684-10%_4.sld, and WEH684-10%_5.sld
File: WEH696_Archive.zip
Description: Time-lapse imaging data of homozygous atg-16.2; atg-16.1 double mutant embryos with green membrane degraded in somatic cells and red histones
Genotype: atg-16.2(ok3224) xnIs390[pie-1::GFP::ZF1::PH(PLC1delta1), unc-119(+)] II; unc-119(ed3) III; Is[mCherry::HistoneH2B] IV; atg-16.1(gk668615[Q356Stop]) X
Contains WEH696-10%.sld and WEH696-10%_2.sld
File: WEH700_Archive.zip
Description: Time-lapse imaging data of wild type control embryos with green membrane and red histones degraded in somatic cells
Genotype: wurIs144[pGF13: pie-1::ZF1::mCherry::his-15; unc-119(+)] I; unc-119(ed3) ltIs38[pie-1::GFP::PH(PLC1delta1), unc-119(+)] III
Contains WEH700-10%.sld, WEH700-10%-2c.sld, WEH700-10%-2c2.sld, WEH700-10%-2c3.sld, WEH700-10%-2c4.sld, WEH700-10%-2c5.sld, WEH700-10%-2c6.sld, WEH700-10%-2c7.sld, WEH700-10%-3c.sld, WEH700-10%-3c2.sld, WEH700-10%-4c.sld, WEH700-10%-4c2.sld, and WEH700-10%-4c3.sld
File: WEH708_Archive.zip
Description: Time-lapse imaging data of atg-16.2 mutant embryos with green membrane and red histones degraded in somatic cells
Genotype: wurIs144[pGF13: pie-1::ZF1::mCherry::his-15; unc-119(+)] I; atg-16.2(gk145022[W253Stop]) II; unc-119(ed3) ltIs38[pie-1::GFP::PH(PLC1delta1), unc-119(+)] III
Contains WEH708-10%.sld and WEH708-10%_2.sld
File: WEH714_Archive.zip
Description: Time-lapse imaging data of homozygous atg-16.2; atg-16.1 double mutant embryos with green membrane and red histones degraded in somatic cells
Genotype: wurIs144[pGF13: pie-1::ZF1::mCherry::his-15; unc-119(+)] I; atg-16.2(gk145022[W253Stop]) II; unc-119(ed3) ltIs38[pie-1::GFP::PH(PLC1delta1), unc-119(+)] III; atg-16.1(gk668615[Q356Stop]) X
Contains WEH714-10%.sld, WEH714-10%_2.sld, and WEH714-10%_3.sld
File: WEH722_Archive.zip
Description: Time-lapse (10% fluorescence) and still (50% fluorescence) imaging data of wild type control embryos with green histones and red LC3 homolog LGG-2
Genotype: Si[pVIG57: Pmex-5::mCherry::LGG-2::tbb-2 3’UTR, C.b. unc-119(+)] II; unc-119(ed3) ruIs32[pAZ132: pie-1::GFP::H2B, unc-119(+)] III
Contains WEH722-10%.sld, WEH722-10% 1 cell movies.sld, and WEH722-50%.sld
File: WEH728_Archive.zip
Description: Still images of atg-16.2 mutant embryos with green histones and red LC3 homolog LGG-2
Genotype: Si[pVIG57: Pmex-5::mCherry::LGG-2::tbb-2 3’UTR, C.b. unc-119(+)] atg-16.2(gk145022[W253Stop]) II; unc-119(ed3) ruIs32[pAZ132: pie-1::GFP::H2B, unc-119(+)] III
Contains WEH728-50%.sld
File: WEH729_Archive.zip
Description: Still images of atg-9 mutant embryos with green histones and red LC3 homolog LGG-2
Genotype: Si[pVIG57: Pmex-5::mCherry::LGG-2::tbb-2 3’UTR, C.b. unc-119(+)] II; unc-119(ed3) ruIs32[pAZ132: pie-1::GFP::H2B, unc-119(+)] III; atg-9(bp564) V
Contains WEH729-50%.sld
File: WEH731_Archive.zip
Description: Time-lapse imaging data of atg-9 mutant embryos with green membrane and red histones degraded in somatic cells
Genotype: wurIs144[pGF13: pie-1::ZF1::mCherry::his-15; unc-119(+)] I; unc-119(ed3) ltIs38[pie-1::GFP::PH(PLC1delta1), unc-119(+)] III; atg-9(bp564) V
Contains WEH731-10%.sld, WEH731-10%-2.sld, WEH731-10% 2 hr.sld, WEH731-10% 2 hr2.sld, WEH731-10% 2 hr3.sld, WEH731-10% 2 hr-2c9.sld, WEH731-10% 2 hr-2c10.sld, and WEH731-10% 2 hr-3c.sld
File: WEH734_Archive.zip
Description: Still images of atg-16.1 mutant embryos with green histones and red LC3 homolog LGG-2
Genotype: Si[pVIG57: Pmex-5::mCherry::LGG-2::tbb-2 3’UTR, C.b. unc-119(+)] II; unc-119(ed3) ruIs32[pAZ132: pie-1::GFP::H2B, unc-119(+)] III; atg-16.1(gk668615[Q356Stop]) X
Contains WEH734-50%.sld
File: WEH739_Archive.zip
Description: Time-lapse (10% fluorescence) and still (50% fluorescence) imaging data of homozygous atg-16.2; atg-16.1 double mutants with green histones and red LC3 homolog LGG-2
Genotype: Si[pVIG57: Pmex-5::mCherry::LGG-2::tbb-2 3’UTR, C.b. unc-119(+)] atg-16.2(gk145022[W253Stop]) II; unc-119(ed3) ruIs32[pAZ132: pie-1::GFP::H2B, unc-119(+)] III; atg-16.1(gk668615[Q356Stop]) X
Contains WEH739-2 cell movies 10%.sld and WEH739-50%.sld
File: WEH755_Archive.zip
Description: Still images of wild type control embryos with green histones and red LC3 homolog LGG-2 degraded in blastomeres after the first mitotic division
Genotype: wurSi2[pVIG57-CTPD: Pmex-5::CTPD::mCherry::LGG-2::tbb-2 3’UTR, C.b. unc-119(+)] II; unc-119(ed3) ruIs32[pAZ132: pie-1::GFP::H2B, unc-119(+)] III
Contains WEH755-50%-1s exposure red.sld
Code/software
SlideBook Reader software
https://go.intelligent-imaging.com/get-slidebook-reader
SlideBook Bio-Formats plugin in FIJI or ImageJ software
Instructions on how to add SlideBook access to the Bio-Formats plugin can be found on the 3i website below
https://www.intelligent-imaging.com/technical-answers
Access information
Data was derived from the following sources:
- Imaging data generated in the Wehman Lab at the University of Denver (now relocated to Texas A&M University)
Gravid C. elegans hermaphrodites were dissected in egg salts (94 mM NaCl, 32 mM KCl, 2.8 mM MgCl2, 2.8 mM CaCl2, 2 mM HEPES, pH 7.5) to isolate embryos and mounted on a 4% agarose pad for live imaging. Z-stacks were collected using a Zeiss Axio Observer 7 inverted microscope with Plan-APO 40X 1.4 NA oil objective with Excelitas Technologies X-Cite 120LED Boost illumination, and Hamamatsu ORCA-Fusion sCMOS camera controlled by 3i SlideBook6 software. Time-lapse imaging was acquired sequentially for mCherry and GFP every minute. Data is provided in the SlideBook format (.sld).