1. Cell Biology
  2. Immunology and Inflammation

A selective LIS1 requirement for mitotic spindle assembly discriminates distinct T-cell division mechanisms within the T-cell lineage

  1. Jérémy Argenty
  2. Nelly Rouquié
  3. Cyrielle Bories
  4. Suzanne Mélique
  5. Valérie Duplan-Eche
  6. Abdelhadi Saoudi
  7. Nicolas Fazilleau
  8. Renaud Lesourne  Is a corresponding author
  1. Toulouse Institute for Infectious and Inflammatory Diseases (Infinity), INSERM UMR1291, CNRS UMR5051, University Toulouse III, France
https://doi.org/10.7554/eLife.80277
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Cite this article
  1. Jérémy Argenty
  2. Nelly Rouquié
  3. Cyrielle Bories
  4. Suzanne Mélique
  5. Valérie Duplan-Eche
  6. Abdelhadi Saoudi
  7. Nicolas Fazilleau
  8. Renaud Lesourne
(2022)
A selective LIS1 requirement for mitotic spindle assembly discriminates distinct T-cell division mechanisms within the T-cell lineage
eLife 11:e80277.
https://doi.org/10.7554/eLife.80277
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7 figures, 3 videos, 1 table and 1 additional file

Figures

Figure 1 with 1 supplement
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LIS1 is required for T-cell development following the β-selection checkpoint.

Phenotypic analyses of thymocytes from control and CD2-Lis1 cKO mice. (A) Dot plots show CD4 versus CD8 surface staining on thymocytes from control and CD2-Lis1 cKO mice. Histogram bars represent the numbers of thymocytes in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent a pool of four independent experiments each including n = 3–4 mice per group. (B) Dot plots show CD44 versus CD25 surface staining on CD4-CD8- [DN] thymocytes from control and CD2-Lis1 cKO mice. Histogram bars represent the numbers of thymocytes in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent a pool of five independent experiments each including n = 4–5 mice per group. (C) Dot plots show CD27 versus TCRβ intracellular staining on DN3 thymocytes from control and CD2-Lis1 cKO mice. Histogram bars represent the percentages of TCRβhiCD27hi thymocytes in DN3 thymocytes. Data are mean ± SD and represent a pool of two independent experiments each including n = 2–3 mice per group. (D) Dot plots show CD5 versus TCRβ intracellular staining on DN3 thymocytes from control and CD2-Lis1 cKO mice. Histogram bars represent the percentages of TCRβhiCD5hi thymocytes in DN3 thymocytes and the MFI of TCRβ and CD5 in DN3 TCRβhiCD5hi thymocytes from mice of the indicated genotype. Data are mean ± SD and represent a pool of two independent experiments each including n = 3 mice per group. (E) Histogram graphs show IL-7R, CD71 surface staining and forward-scatter (FSC) on DN3 thymocytes expressing the TCRβ chain. Histogram bars represent the MFI of IL-7R, CD71, and FSC in the indicated DN3 thymocytes subsets. Data are mean ± SD and represent a pool of two independent experiments each including n = 3 mice per group. (F) Histogram graphs show DNA intracellular staining on DN3 thymocytes from the indicated subsets. The percentages represent cells in the G2/M phase of cell cycle. Histogram bars represent the percentages of DN3 TCRβhiCD5hi thymocytes in the G2/M phase of cell cycle. Data are mean ± SD and represent a pool of three independent experiments each including n = 1 mouse per group. Unpaired two-tailed Mann–Whitney t tests were performed for all analyses. **p<0.01; ***p<0.001; ****p<0.0001.

Figure 1—source data 1

LIS1 is required for T-cell development following the β-selection checkpoint.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig1-data1-v2.zip
Figure 1—figure supplement 1
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LIS1 is required for B-cell development and is effective at single-gene dosage during T-cell development.

(A) Dot plots show TCR versus B220 and CD4 versus CD8 surface staining on splenocytes from control and CD2-Lis1 cKO mice. Histogram bars represent the numbers of thymocytes in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent four independent experiments each including n = 3–4 mice per group. (B) Dot plots show CD4 versus CD8 surface staining on total thymocytes and CD44 versus CD25 surface staining on CD4-CD8- [DN] thymocytes from control (Pafah1b1flox/+) and CD2-Lis1 cKO-het mice. Histogram bars represent the percentages of thymocytes in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent a pool of two independent experiments each including n = 1–2 mice per group. (C) Upper dot plots show B220 versus CD19 on bone marrow cells from control and CD2-Lis1 cKO mice. Lower dot plots show IgM versus c-Kit staining on B220+CD19+ bone marrow cells from control and CD2-Lis1 cKO mice. Histogram bars represent the numbers of cells in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent two independent experiments each including n = 3–4 mice per group. Unpaired two-tailed Mann–Whitney t tests were performed. *p<0.05; **p<0.01; ***p<0.001; ****p<0.0001.

Figure 1—figure supplement 1—source data 1

LIS1 is required for B-cell development and is effective at single-gene dosage during T-cell development.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig1-figsupp1-data1-v2.zip
Figure 2
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LIS1 is required for the proliferation of immature thymocytes after the β-selection checkpoint.

(A) CD5lo DN3 thymocytes from control and CD2-Lis1 cKO mice were stained with CellTrace violet (CTV) and stimulated with OP9-Dl1 cells for 48 or 72 hr. The histogram graph shows CTV dilution. Bar graphs represent the proliferation of cells determined by flow cytometry at 24, 48, and 72 hr after stimulation. Data are mean ± SD and represent 3–7 independent experiments each including n = 1–2 pooled mice per group. (B) CD5lo DN3 thymocytes from control and CD2-Lis1 cKO mice were stimulated with OP9-Dl1 cells for the indicated periods of time. Dot plots show CD44 versus CD25 surface staining on thymocytes from control and CD2-Lis1 cKO mice. Data are representative of three independent experiments each including n = 1–2 pooled mouse per group. (C) CD71lo DN3 thymocytes from control and CD2-Lis1 cKO were stimulated with OP9-Dl1 cells for 24 hr. Dot plots show CD5 versus TCRβ intracellular staining on thymocytes. Histogram bars represent the percentages of TCRβhiCD5hi thymocytes in DN3 thymocytes and the MFI CD5 in DN3 TCRβhiCD5hi thymocytes from mice of the indicated genotype. Data are mean ± SD and represent four independent experiments each including n = 1–2 pooled mice per group. (D) CD71lo DN3 thymocytes from control and CD2-Lis1 cKO mice were stimulated with OP9-Dl1 cells for 48 hr. Dot plots show CD5 versus CD71 staining on CTVhi thymocytes. Histogram bars represent the percentages of CD71hiCD5hi thymocytes in CTVlo DN3 thymocytes. Data are mean ± SD and represent four independent experiments each including n = 1–2 pooled mice per group. (E) CD71lo DN3 thymocytes from control and CD2-Lis1 cKO mice were stimulated with OP9-Dl1 cells for 24 hr. The histogram graph shows BCL-2 intracytoplasmic staining in TCRβloCD5lo and TCRβhiCD5hi thymocyte subsets. Histogram bars represent the MFI of BCL-2 in the indicated DN3 thymocyte subsets. Data are mean ± SD and represent three independent experiments each including n = 1–2 pooled mice per group. (F) CD71lo DN3 thymocytes from control and CD2-Lis1 cKO mice were stimulated with OP9-Dl1 cells for 48 hr. Histogram graphs show DNA intracellular staining on thymocytes from the indicated DN3 subsets. The indicated percentages represent cells in the G2/M phase of cell cycle. Histogram bars represent the percentages of DN3 TCRβhiCD5hi thymocytes in the G2/M phase of cell cycle. Data are mean ± SD and represent six independent experiments each including n = 1–2 pooled mice per group. (A) Unpaired two-tailed Welch t tests were performed. (C–E) Unpaired two-tailed Mann–Whitney t tests were performed. *p<0.05, **p<0.01.

Figure 2—source data 1

LIS1 is required for the proliferation of immature thymocytes after the β-selection checkpoint.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig2-data1-v2.zip
Figure 3 with 2 supplements
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LIS1 is required for the proliferation of CD4+ T cells in response to antigen stimulation.

(A) CD4+ T cells from control and CD4-Lis1 cKO mice were stained with CellTrace violet (CTV) and stimulated with anti-CD3 and anti-CD28 antibodies or with phorbol 12-myristate 13-acetate (PMA) and ionomycin (P/I) for 72 hr. The histogram graphs show CTV dilution. Bar graphs represent the percentages of cells that divided at least one-time (Tot.) or that divided one, two, or three times (D1, D2, D3) as determined by flow cytometry at 72 hr after stimulation. Data are mean ± SD and represent five independent experiments each including n = 3 mice per group. (B) CD4+ T cells from control and CD4-Lis1 cKO mice were stimulated with anti-CD3 and anti-CD28 antibodies for 24 hr. Bar graphs represent the percentages of cells expressing CD25 and CD69 as determined by flow cytometry. Data are mean ± SD and represent two independent experiments each including n = 1–2 mice per group. (C) CD4+ and CD8+ T cells from control and CD4-Lis1 cKO mice were stimulated with anti-CD3 and anti-CD28 antibodies for 48 hr. Histogram graphs show DNA intracellular staining on CD4+ and CD8+ T cells. The indicated percentages represent cells in the G2/M phase of cell cycle. Histogram bars represent the percentages of CD4+ and CD8+ T cells in the G2/M phase of cell cycle. Data are mean ± SD and represent two independent experiments each including n = 3 mice per group. (D) CD8+ T cells from control and CD4-Lis1 cKO mice were stained with CTV and stimulated with anti-CD3 and anti-CD28 antibodies or with PMA and ionomycin (P/I) for 72 hr. The histogram graph shows CTV dilution. Bar graphs represent the percentages of cells that divided at least one-time (Tot.) or that divided one, two,or three times (D1, D2, D3) as determined by flow cytometry at 72 hr after stimulation. (E, F) C57BL/6j mice (CD45.2+) were injected i.v. with CTV-stained CD45.1+CD4+ T cells from OT2 and OT2 CD4-Lis1 cKO mice. Mice were then immunized with ovalbumin emulsified in RIBI. Proliferation of CD45.1+CD4+T cells was analyzed at days 2 and 3 after immunization. (E) Bar graphs represent the proliferation and numbers of CD45.1+CD4+T cells as determined by flow cytometry at days 2 and 3 after immunization. Data are mean ± SD and are representative of one experiment out of two independent experiments each including n = 5 mice per group. (F) The histogram graph shows CTV dilution in CD45.1+CD4+T cells at day 3 after immunization. Histograms overlay shows CD44 surface staining on undivided CD45.1+CD4+T cells at day 3 after immunization. Data are representative of one experiment out of two independent experiments each including n = 5 mice per group. Unpaired two-tailed Mann–Whitney t tests were performed for all analyses. *p<0.05; **p<0.01; ***p<0.001; ****p<0.0001.

Figure 3—source data 1

LIS1 is required for the proliferation of CD4+ T cells in response to antigen stimulation.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig3-data1-v2.zip
Figure 3—figure supplement 1
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Normal T-cell development in CD4-Lis1 cKO mice.

Phenotypic analyses of thymocytes from control and CD4-Lis1 cKO mice. (A) Dot plots show CD4 versus CD8 surface staining on thymocytes from control and CD4-Lis1 cKO mice. Histogram bars represent the numbers of thymocytes in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent two independent experiments each including n = 2–3 mice per group. (B) Dot plots show CD24 versus TCRβ surface staining on CD4+ SP and CD8+ SP thymocytes from control and CD4-Lis1 cKO mice. Histogram bars represent the numbers of thymocytes in the indicated subset from mice of the indicated genotype. Data are mean ± SD and represent two independent experiments each including n = 2 mice per group. (C) Dot plots show CD4 versus CD8 surface staining on thymocytes from control and CD4-Lis1 cKO mice expressing the AND TCR transgene. Histogram graphs represent the TCR Vα11 surface staining on total thymocytes. Histogram bars represent the numbers of thymocytes in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent two independent experiments each including n = 2–3 mice per group. (D) Dot plots show TCR versus B220 and CD4 versus CD8 surface staining on total splenocytes and splenic T cells, respectively, from control and CD4-Lis1 cKO mice. Histogram bars represent the numbers of cells in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent two independent experiments each including n = 2–3 mice per group. (E) Dot plots show CD4 versus CD8 surface staining on splenocytes from control (pagah1b1flox/+) and CD4-Lis1 cKO-het mice. Histogram bars represent the numbers of cells in each indicated subset from mice of the indicated genotype. Data are mean ± SD and represent two independent experiments each including n = 3–4 mice per group. *p<0.05; **p<0.01; ***p<0.001; ****p<0.0001.

Figure 3—figure supplement 1—source data 1

Normal T-cell development in CD4-Lis1 cKO mice.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig3-figsupp1-data1-v2.zip
Figure 3—figure supplement 2
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Effect of LIS1 haploid and diploid deficiency on CD4+ T-cell proliferation and expansion.

(A) CD4+ T cells from control (Pafah1flox/+) and CD4-Lis1 cKO-het were stained with CellTrace violet (CTV) and stimulated with anti-CD3 and anti-CD28 antibodies for 48 hr. The histogram graphs show CTV dilution. Bar graphs represent the percentages of cells that divided at least one-time (Tot.) or that divided one, two, or three times (D1, D2, D3) as determined by flow cytometry at 72 hr after stimulation. Data are mean ± SD and represent two independent experiments each including n = 4 mice per group. (B) Total cytoplasmic extracts of CD4+ and CD8+ T cells from control and CD4-Lis1 cKO mice were analyzed by Western blotting with antibodies against LIS1 and GAPDH, the loading control. (C) Bar graphs represent the percentages and numbers of CD45.1+CD4+ T cells as determined by flow cytometry at day 7 after immunization. Data are mean ± SD and are representative of one experiment including n = 5 mice per group. **p<0.01.

Figure 3—figure supplement 2—source data 1

Effect of LIS1 haploid and diploid deficiency on CD4+ T-cell proliferation and expansion.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig3-figsupp2-data1-v2.zip
Figure 4
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Dysfunctional chromosome alignment in LIS1-deficient CD4+ T cells leads to abortive mitosis and aneuploidy.

(A) CD4+ T cells from control and CD4-Lis1 cKO mice were stimulated with anti-CD3 and anti-CD28 antibodies for 48 hr. Histogram graphs represent the Bright Detail Intensity (BDI) feature on CD4+ T cells in the G2/M phase as determined by image stream flow cytometry. Numbers represent the percentages of cells in mitosis according to the BDI feature. Images represent DAPI staining in BDIlow and BDIhi control CD4+ T cells. Bar graphs represent the percentages of cells in mitosis (M) out of cells in the G2/M phase (n = 30,000 cells). Data are mean ± SD and represent three independent experiments each including n = 1 mouse per group. (B) CD4+ T cells from control and CD4-Lis1 cKO mice were stimulated with anti-CD3 and anti-CD28 antibodies for 24 hr, synchronized with nocodazole for 18 hr and incubated with MG132 for 3 hr to induce metaphase arrest. Histogram graphs represent the Elongatedness feature on CD4+ T cells in the M phase as determined by image stream flow cytometry. Numbers represent the percentages of cells in metaphase according to Elongatedness feature (n = 30,000 cells). Images represent DAPI staining in Elongatednesslow and Elongatednesshi control CD4+ T cells. Bar graphs represent the percentages of cells in metaphase out of cells in the M phase. Data are mean ± SD and represent three independent experiments each including n = 1 mouse per group. (C) Time-lapse microscopy analysis of cell division in CD4+ T cells from control and CD4-Lis1 cKO mice stimulated with anti-CD3 and anti-CD28 antibodies. Images represent DNA staining on CD4+ T cells at the indicated times (hours:minutes). White arrows represent cells with uncondensed DNA. Red arrows represent the same cells after chromosomes formation. The top red arrows in the CD4-Lis1 cKO panel are representative of abortive mitosis. The bottom red arrows in the CD4-Lis1 cKO panel are representative of mitosis leading to aneuploidy. Bar graphs represent the time of mitosis per cell. Data are mean ± SD and represent three independent experiments each including n = 1 mouse per group. (D) Mitosis outcomes in control and CD4-Lis1 cKO CD4+ T cells stimulated with anti-CD3 and anti-CD28 antibodies. Numbers represent percentages in the different section out of a total of n = 62–64 mitosis analyzed. Data represent three independent experiments each including n = 1 mouse per group. (E) CD4+ T cells from control and CD4-Lis1 cKO mice were stimulated with anti-CD3 and anti-CD28 antibodies for 48 hr. Cells in G2 phase were analyzed by image stream flow cytometry. Cells stained with DAPI and bright-field (BF) images are represented. Bar graphs represent the percentages of cells with multilobed nuclei (n = 400 cells). Data are mean ± SD and represent three independent experiments each including n = 1 mouse per group. (A, B) Unpaired two-tailed Welch t tests were performed. (C) Unpaired two-tailed Mann–Whitney t test was performed. *p<0.05; **p<0.01; ***p<0.001; ****p<0.0001.

Figure 4—source data 1

Dysfunctional chromosome alignment in LIS1-deficient CD4+ T cells leads to abortive mitosis and aneuploidy.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig4-data1-v2.zip
Figure 5
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Proliferation leads to p53 upregulation and apoptosis in LIS1-deficient thymocytes and CD4+ T cells.

(A) CD4+ T cells from control and CD4-Lis1 cKO mice were stained with CellTrace violet (CTV) and stimulated with anti-CD3 and anti-CD28 antibodies for 48 hr. The histogram graphs show annexin-5 staining on CTVhi (top panel) and CTVlow (bottom panel) CD25+CD4+T cells. Bar graphs represent the percentages of annexin5+ cells in the indicated subsets. Data are mean ± SD and represent two independent experiments each including n = 1–2 mice per group. (B) Total CD4+ and CD8+ T cells from control and CD4-Lis1 cKO mice were stimulated with anti-CD3 and anti-CD28 antibodies for the indicated times. Total cytoplasmic extracts of the cells were then analyzed by Western blotting with antibodies against p53, Rac1, and GAPDH, the loading controls. Data are representative of two independent experiments. (C) CD5lo DN3 thymocytes from control and CD2-Lis1 cKO mice were stained with CTV and stimulated with OP9-Dl1 cells for 48 hr. The histogram graphs show annexin-5 staining on CTVhi (top panel) and CTVlow (bottom panel) CD5hiCD4+ T cells. Bar graphs represent the percentages of annexin5+ cells in the indicated subsets. Data are mean ± SD and represent two independent experiments each including n = 2 mice per group. (D) Total cytoplasmic extracts of the DN thymocytes were analyzed by Western blotting with antibodies against p53 and Rac1, the loading control. Data are representative of two independent experiments. Unpaired two-tailed Welch t tests were performed in (A, C). *p<0.05; ***p<0.001.

Figure 5—source data 1

Proliferation leads to p53 upregulation and apoptosis in LIS1-deficient thymocytes and CD4+ T cells.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig5-data1-v2.zip
Figure 6
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Impaired formation of dynein/dynactin complexes is associated with the loss of centrosome integrity and the formation of multipolar spindles in LIS-1-deficient thymocytes and CD4+ T cells.

(A) CD4+ T cells from control and CD4-Lis1 cKO mice were stained with CellTrace violet (CTV) and stimulated with anti-CD3 and anti-CD28 antibodies for 48 hr. Images represent maximum intensity projection of γ-tubulin and DAPI staining on undivided FSClo (top panel) and FSChi (bottom panel) CD4+ T cells. Bar graphs represent the percentages of cells with the indicated number of centrosome in total cells (top graph) or in mitotic cells (bottom graph). Data represent one experiment out of two independent experiments with n = 30–50 cells analyzed per group. (B) CD4+ T cells from control and CD4-Lis1 cKO mice were stained with CTV and stimulated with anti-CD3 and anti-CD28 antibodies for 48 hr. Images represent maximum intensity projection of γ-tubulin and α-tubulin staining on undivided FSChi CD4+ T cells. Bar graphs represent the size of the pericentriolar region (PCM) based on γ-tubulin staining in mitotic cells with the indicated number of centrosomes. Data represent three experiments with n = 16–54 centrosomes analyzed per group. (C) Images represent maximum intensity projection of γ-tubulin and DAPI staining CD5hi DN3 thymocytes. Bar graphs represent the percentages of cells with the indicated number of centrosomes in mitotic cells. Data represent one experiment out of two independent experiments with n = 30–50 cells analyzed per group. (D) CD4+ T cell extracts from control and CD4-Lis1 cKO mice were subjected to immunoprecipitation (IP) with antibodies specific of the intermediate chain of dynein (DIC) or with an IgG2b isotype control and then analyzed by Western blotting with antibodies specific of the indicated proteins (dynein heavy chain [DHC]). Data represent one experiment out of two independent experiments. Unpaired two-tailed Mann–Whitney t test was performed. ****p<0.0001.

Figure 6—source data 1

Impaired formation of dynein/dynactin complexes is associated with the loss of centrosome integrity and the formation of multipolar spindles in LIS-1 deficient thymocytes and CD4+ T cells.

https://cdn.elifesciences.org/articles/80277/elife-80277-fig6-data1-v2.zip
Author response image 1
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KI67 expression profile in thymocytes from Lis1flox/flox and CD2-Cre Lis1flox/flox mice.

Left panel. Histogram overlay represent KI67 staining on DN3-CD5hi thymocytes from Lis1flox/flox and CD2-Cre Lis1flox/flox mice. Middle panel. Histograms represent KI67 staining on the indicated thymocyte subsets from Lis1flox/flox (WT) mice. Right panel. Dot plot represent CD5 versus Ki67 staining on DN3 thymocytes.

Videos

Video 1
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Time-lapse microscopy of mitosis in wild-type CD4+ T cells.

Time-lapse microscopy analysis of mitosis in CD4+ T cells from wild-type mice stimulated with anti-CD3 and anti-CD28 antibodies. Videos represent DNA staining (right panel) and bright field (left panel) on CD4+ T cells.

Video 2
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Time-lapse microscopy of abortive mitosis in Lis1-deficient CD4+ T cells.

Time-lapse microscopy analysis of mitosis in CD4+ T cells from CD4-Lis1 cKO mice stimulated with anti-CD3 and anti-CD28 antibodies. Videos represent DNA staining (right panel) and bright field (left panel) on CD4+ T cells.

Video 3
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Time-lapse microscopy of mitosis with aneuploidy in Lis1-deficient CD4+ T cells.

Time-lapse microscopy analysis of mitosis in CD4+ T cells from CD4-Lis1 cKO mice stimulated with anti-CD3 and anti-CD28 antibodies. Videos represent DNA staining (right panel) and bright field (left panel) on CD4+ T cells.

Tables

Key resources table
Reagent type (species) or resourceDesignationSource or referenceIdentifiersAdditional information
Genetic reagent
(Mus musculus)		129S-Pafah1b1tm2Awb/JJackson LaboratoriesStrain #:008002;
RRID:IMSR_JAX:008002		This stain was provided by Dr. Deanna S. Smith (University of South Carolina, Columbia, USA)
Genetic reagent
(Mus. musculus)		B6.Cg-Tg(CD2-icre)4Kio/JJackson LaboratoriesStrain #:008520;
RRID:IMSR_JAX:008520
Genetic reagent
(M. musculus)		Tg(Cd4-cre)1Cwi/BfluJJackson LaboratoriesStrain #:017336;
RRID:IMSR_JAX:017336
Cell line 
(M. musculus)		OP9-dl1Schmitt et al., 2004Provided by Dr. Sophie Laffont Pradines (Toulouse Institute for Infectious and Inflammatory Diseases, Toulouse France)
AntibodyAnti-CD3ε
(hamster monoclonal)		BioLegendClone 2C-11Purified unconjugated
AntibodyAnti-CD28
(hamster monoclonal)		BioLegendClone 37.51Purified unconjugated
AntibodyAnti-CD8α
(rat monoclonal)		Thermo Fisher ScientificClone 53-6.7Conjugated to A-700
(1/300)
AntibodyAnti-CD4
(rat monoclonal)		BD BiosciencesClone RM4-5Conjugated to Pacific Blue (1/1000)
AntibodyAnti-CD24
(rat monoclonal)		BioLegendClone M1/69Conjugated to PE
(1/500)
AntibodyAnti-TCRβ
(hamster monoclonal)		BD BiosciencesClone H57-597Conjugated to
FITC
(1/400)
AntibodyAnti-TCRβ
(hamster monoclonal)		Thermo Fisher ScientificClone H57-597Conjugated to
PECy7
(1/1500)
AntibodyAnti-Vα11
(rat monoclonal)		BD BiosciencesClone RR8-1Conjugated to
FITC
(1/400)
AntibodyAAnti-CD5
(rat monoclonal)		BD BiosciencesClone 53-7.3Conjugated to
APC
(1/1000)
AntibodyAnti-CD5
(rat monoclonal)		Thermo Fisher ScientificClone 53-7.3Conjugated to
FITC
(1/1000)
AntibodyAnti-CD69
(hamster monoclonal)		BD BiosciencesClone H1.2F3Conjugated to
FITC
(1/200)
AntibodyAnti-B220
(rat monoclonal)		BD BiosciencesClone RA3-6B2Conjugated to
PE
(1/400)
AntibodyAnti-Gr1
(rat monoclonal)		BioLegendClone RB6-8C5Conjugated to
PE
(1/300)
AntibodyAnti-CD11b
(rat monoclonal)		BioLegendClone M1/70Conjugated to
PE
(1/200)
AntibodyAnti-CD11c
(hamster monoclonal)		BioLegendClone N418Conjugated to
PE
(1/200)
AntibodyAnti-Ter119
(rat monoclonal)		BioLegendClone TER119Conjugated to
PE
(1/200)
AntibodyAnti-CD3ε
(hamster monoclonal)		BioLegendClone 145-2C11Conjugated to
PE
(1/200)
AntibodyAnti-NK1.1
(mouse monoclonal)		BD BiosciencesClone PK136Conjugated to
PE
(1/200)
AntibodyAnti-TCRγδ
(hamster monoclonal)		BD BiosciencesClone GL3Conjugated to
(1/200)
AntibodyAnti-CD44
(rat monoclonal)		Thermo Fisher ScientificClone IM7Conjugated to
FITC
(1/200)
AntibodyAnti-CD25
(rat monoclonal)		BD BiosciencesClone PC61.5Conjugated to
PercP Cy5.5
(1/300)
AntibodyAnti-CD71
(rat monoclonal)		BioLegendClone R17217Conjugated to
PeCy7
(1/400)
AntibodyAnti-CD27
(hamster monoclonal)		BD BiosciencesClone LG.3A10Conjugated to
APC
(1/200)
AntibodyAnti-IL-7R
(rat monoclonal)		BD BiosciencesClone A7R34Conjugated to
A700 (1/500)
AntibodyAnti-IL-7R
(rat monoclonal)		BD BiosciencesClone A7R34Conjugated to
APC (1/400)
AntibodyAnti-BCL-2
(hamster monoclonal)		BD BiosciencesClone 3F11Conjugated to
FITC
(5 μL/105 cells)
AntibodyAnti-CD19
(rat monoclonal)		BioLegendClone 1D3/CD19Conjugated to
PercPCY5.5
(1/500)
AntibodyAnti-c-kit
(rat monoclonal)		BioLegendClone 2B8Conjugated to
PE
(1/200)
AntibodyAnti-c-kit
(rat monoclonal)		BD BiosciencesClone 2B8Conjugated to
APC
(1/200)
AntibodyAnti-IgM
(rat monoclonal)		BD BiosciencesClone RMM-1Conjugated to
PECy7
(1/300)
AntibodyAnti-CD45.1
(mouse monoclonal)		BD BiosciencesClone A20Conjugated to
PE
(1/500)
AntibodyAnti-γ-tubulin
(mouse monoclonal)		BioLegendClone 14C11Purified unconjugated
AntibodyAnti-α-tubulin
(mouse monoclonal)		Thermo Fisher ScientificClone DM1APurified unconjugated
AntibodyGoat anti-mouse IgG2bThermo Fisher ScientificCat#A-21147Alexa Fluor 555
AntibodyAnti-Dynein IC
(mouse monoclonal)		Santa Cruz BiotechnologiesClone 74-1Purified unconjugated
AntibodyAnti-LIS1
(rabbit polyclonal)		Santa Cruz Biotechnologiessc-15319Purified unconjugated
AntibodyAnti-Dynein HC
(rabbit polyclonal)		Santa Cruz Biotechnologiessc-9115Purified unconjugated
AntibodyAnti-p150glued
(mouse monoclonal)		BD BiosciencesClone 1/p150GluedPurified unconjugated
AntibodyAnti-p53
(mouse monoclonal)		Cell SignalingClone 1C12Purified unconjugated
AntibodyAnti-Rac1
(mouse monoclonal)		MilliporeClone 23A8Purified unconjugated
OtherAnnexinVBD BiosciencesRRID:AB_2868885APC
(5 µL/105 cells)
OtherAnnexinV binding bufferBD BiosciencesCat#556454Used for annexinV staining
OthereBioscience Fixable Viability DyeThermo Fisher ScientificCat#65-0865-14eFluor 780
APC-H7
OtherPermeabilization bufferThermo Fisher ScientificCat#00-8333-56Used for intracytoplasmic staining
OtherChambered glass coverslipIBIDICat#80821Used for videomicroscopy analyses
OtherDynabeads Untouched Mouse CD4 Cells KitThermo Fisher ScientificCat#11415DMagnetic beads used for the purification of CD4-CD8- thymocytes as well as CD4+ and CD8+ T cells
OtherDAPISigma-AldrichCat#D95421 mg/mL
Nuclear staining for microscopy
OtherHoechst 33342Sigma-AldrichCat#1453350 ng/mL
Nuclear staining for videomicroscopy
OtherCell trace VioletThermo Fisher ScientificCat#C345572 μM
Cell tracker used for proliferation analyses
OtherDABCOSigma-AldrichCat#D27802Mounting medium for microscopy
OtherMouse IL-7PeproTechCat#21-–1710 ng/mL
Chemical compound, drugNocodazoleSigma-AldrichCat#M1404100 ng/mL
Inhibitor of microtubule polymerization
Chemical compound, drugMG132Sigma-AldrichCat#M744910 μM
proteasome inhibitor
Chemical compound, drugPhorbol 12-myristate 13-acetate (PMA)Sigma-AldrichCat#P8139100 ng/ml
T-cell pharmacological stimulator
Chemical compound, drugIonomycinSigma-AldrichCat#I0634100 ng/ml
T-cell pharmacological stimulator
Chemical compound, drugRIBISigma Adjuvant SystemCat#S6322Adjuvant
Software, algorithmIDEASMillipore

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https://cdn.elifesciences.org/articles/80277/elife-80277-mdarchecklist1-v2.pdf

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  1. Jérémy Argenty
  2. Nelly Rouquié
  3. Cyrielle Bories
  4. Suzanne Mélique
  5. Valérie Duplan-Eche
  6. Abdelhadi Saoudi
  7. Nicolas Fazilleau
  8. Renaud Lesourne
(2022)
A selective LIS1 requirement for mitotic spindle assembly discriminates distinct T-cell division mechanisms within the T-cell lineage
eLife 11:e80277.
https://doi.org/10.7554/eLife.80277