bj 5ta fibroblasts (ATCC)
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Bj 5ta Fibroblasts, supplied by ATCC, used in various techniques. Bioz Stars score: 96/100, based on 463 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/bj+5ta+fibroblasts/bio_rxiv__64898__2026__05__04__722669-163-15-20?v=ATCC
Average 96 stars, based on 463 article reviews
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1) Product Images from "Loss of MTPAP disrupts mitochondrial RNA processing causing upregulation of type I interferon signalling"
Article Title: Loss of MTPAP disrupts mitochondrial RNA processing causing upregulation of type I interferon signalling
Journal: bioRxiv
doi: 10.64898/2026.05.04.722669
Figure Legend Snippet: A-B: Western blot showing levels of MTPAP and mitochondrial complex I (CI) NDUFB8, II (CII) SDHB, III (CIII) CYTB, IV (CIV) COX2, V (CV) ATP5B proteins in lysates of fibroblasts from patient P3, P4 and P5 compared to fibroblasts from 3 healthy donor (controls) ( A ), and in lysates of BJ-5ta deleted for MTPAP by CRISPR/Cas9 using 3 different single guides (sg#1, #2, #3) compared to controls ( B ). Vinculin is used as a loading control. Image representative of 3 different experiments. C: Left, representative confocal images of the mitochondrial network stained with mitochondrial outer membrane protein TOMM40 antibody in patient fibroblasts (P3, P4 and P5) and one healthy donor fibroblast (control). Scale bar: 5 µm. Right, quantification of the mitochondrial footprint based on MiNA ImageJ analysis plugin in patient fibroblasts and the average of 3 healthy donor fibroblasts (control), represented as a superplot (each border free-point represents the measure of a cell, each colour is a different experiment). Mean ± SEM of 3 experiments; ns indicates non significance in a paired t-test performed on the average value for each experiment. D: As in C for MTPAP_KO (sg#2) and control cells. E: Left, representative spinning disk live images of TMRE signal in patient fibroblasts (P3, P4 and P5) compared to one healthy donor fibroblast (control). Scale bar: 5 µm. Right, quantification of TMRE signal in patient fibroblasts relative to the average of 3 healthy donor fibroblasts (control). Superplot, mean ± SEM; n=3 experiments (each colour is a different experiment); each border-free point represents the measure of a cell; * indicates p<0.05 in paired t-test performed on the average value for each experiment. F: As in E for MTPAP_KO (sg#2) and control cells. G-H: ATP production ( G ) and basal respiration ( H ) measured by Seahorse mito stress assay in MTPAP_KO (average of sg#1, sg#2 and sg#3 data for each experiment) versus control cells. mean ± SEM; n=3 experiments, each colour is a different experiment, * indicates p<0.05 in Mann-Whitney test. I-J: ISG score (median of fold changes of mRNA expression of 6 ISGs, see Methods) ( I ) and IFNB1 mRNA expression ( J ) in MTPAP_KO cells compared to controls measured by qPCR. Mean ± SEM; n=7 experiments; each colour corresponds to KO_MTPAP cells generated using a single guide RNA targeting MTPAP; ** p<0.01 in Kruskall-Wallis with Dunn’s post-hoc test.
Techniques Used: Western Blot, CRISPR, Control, Staining, Membrane, MANN-WHITNEY, Expressing, Generated
Figure Legend Snippet: A-B: ISG score ( A ) and IFNB1 mRNA ( B ) in control and MTPAP_KO (sg#2) cells treated for 10 days with ddC. Mean ± SEM; n=4, each colour is a different experiment; * indicates p<0.05, ** p< 0.01, 2-way ANOVA with Holm-Sidak multiple comparison test. C-D: ISG score ( C ) and IFNB1 mRNA levels ( D ) in BJ-5ta cells double KO IRF3/MTPAP compared to controls. E-F : ISG score ( E ) and IFNB1 mRNA levels ( F ) in MAVS/MTPAP double KO cells compared to controls. G-H : ISG score ( G ) and IFNB1 mRNA levels ( H ) in MDA5/MTPAP double KO cells compared to controls. I-J : ISG score ( I ) and IFNB1 mRNA levels ( J ) in RIG-I/MTPAP double KO cells compared to controls. C-J: Mean ± SEM; n≥4, each colour is a different experiment, KO_MTPAP data are represented by the average of sg#1, sg#2 and sg#3 data; ns indicates non significance, * indicates p<0.05 in Wilcoxon test.
Techniques Used: Control, Comparison
Figure Legend Snippet: A: (Left) Relative levels of mtDNA expressed as the averaged relative levels of MT-CO2 , MT-ND1 and mtDNA D-loop signals and ( Right ) of mtRNA expressed as the averaged relative expression levels of MT-ATP6/8 , MT-ND4 , MT-CO1 , MT-CYTB and MT-ND6 in lysates of control cells and of MTPAP_KO cells (sg#2) treated for 10 days with ddC. Mean ± SEM; n=3 experiments, each colour is a different experiment, ** indicates p<0.01, in two-way ANOVA with Holm-Sidak multiple comparison test. B-C-D-J-L-N: Western blot analysis showing protein levels of MTPAP and IRF3 ( B ), STING ( C ), cGAS ( D ), MAVS ( J ), MDA5 ( L ), RIG-I ( N ), in lysates of double KO cells (sg#2 for MTPAP_KO) compared to controls. Vinculin or cofilin are used as loading controls. Pictures representative of 3 different experiments. E: mRNA levels of IFNB1 measured by qPCR in cGAS/MTPAP and STING/MTPAP double KO BJ-5ta cells compared to controls 24 h after stimulation with transfected HT-DNA (sg#2 for MTPAP_KO). Mean ± SEM; n=3 experiments, each colour is a different experiment, **** indicates p< 0.0001 in two-way ANOVA with Holm-Sidak multiple comparison test. F-H: ISG score measured by qPCR in BJ-5ta cells double KO for STING/MTPAP ( F ) cGAS/MTPAP ( H ) cells compared to controls (sg#2 for MTPAP_KO). Mean ± SEM; n≥4 experiments, each colour is a different experiment, MTPAP_KO using sg#2; ns indicates non significance for Wilcoxon tests. G-I: IFNB1 mRNA expression measured by qPCR in double KO STING/MTPAP ( G ) cGAS/MTPAP ( I ) cells compared to controls (sg#2 for MTPAP_KO). N=4 experiments, each colour is a different experiment; ns indicates non significance for Wilcoxon tests. K-M: IFNB1 mRNA expression levels in MAVS_KO ( K ) and MDA5_KO ( M ) cells compared to BJ-5ta controls when transfected with poly(I:C). Mean ± SEM; n=3 experiments, ** indicates p<0.01, *** p< 0.001 in two-way ANOVA with Holm-Sidak multiple comparison test. O: IFNB1 mRNA expression levels in RIG-I_KO BJ-5ta cells compared to controls Infected with Sendai Virus. Mean ± SEM; n=5, ** indicates p<0.01 in two-way ANOVA with Holm-Sidak multiple comparison test.
Techniques Used: Expressing, Control, Comparison, Western Blot, Transfection, Infection, Virus
Figure Legend Snippet: A: Representative confocal microscopy image of immunostaining with antibody to mitochondrial protein TOMM40 and J2 antibody to dsRNA in control and MTPAP_KO (sg#1) cells. Scale bar: 5 µm. B: Quantification of average pixel intensity of J2 dsRNA signal in mitochondria in control vs MTPAP_KO cells (average of sg#1, #2 and #3). Superplot, mean ± SEM; n=3 experiments; each borderless point represents the measure of a cell; each colour is a different experiment; * indicates p<0.05 in paired t-test performed on the mean value for each experiment. C: Percentage of dsRNA dots in mitochondria with an area over 1 µm 2 in control cells vs MTPAP_KO cells (average of sg#1, #2 and #3). Superplot, mean ± SEM; n=3 experiments; each borderless point represents the measure of a cell; each colour is a different experiment; * indicates p<0.05 in paired t-test performed on the mean value for each experiment. D: Representative confocal microscopy image of immunostaining with antibody to mitochondrial RNA granule protein GRSF1 and dsRNA (J2) in control and MTPAP_KO (sg#2) BJ-5ta cells. Scale bar: 5 µm. E: Representative image of the 3D volume reconstruction of STED images after immunostaining with antibody against mitochondrial protein TOMM40 and dsRNA (J2) in control and MTPAP_KO cells (sg#2). Yellow dots correspond to dsRNA particles detected outside of the mitochondrial network. Scale bar: 3 µm. F: Percentage of dsRNA dots detected outside of the mitochondrial network in control vs MTPAP_KO cells (sg#2). Mean ± SEM; n=3 experiments; each point represents the measure of a cell; each colour is a different experiment; **** indicates p<0.0001 in Mann-Whitney test. G: Quantification of the median volume of dsRNA particles detected inside or outside of the mitochondrial network in MTPAP_KO cells (sg#2). Mean ± SEM; n=3 experiments; each point represents the measure of a cell; each colour is a different experiment; *** indicates p<0.001 in Mann-Whitney test. H: Quantification of mtRNA levels measured by qPCR in cytosolic fractions of control and MTPAP_KO cells (sg#2). Mean ± SEM; n=8 experiments; each colour is a different experiment; ns indicates non significance, ** p< 0.01 in 2-way ANOVA with Holm-Sidak multiple comparison test. I-J: ISG score ( I ) and IFNB1 mRNA expression ( J ) measured by qPCR in MTPAP_KO cells (average of sg#1, sg#2 and sg#3 data for each experiment) treated for 24h with 300 µM DIDS compared to controls. Mean ± SEM; n=4 experiments, each colour is a different experiment; * indicates p<0.05, ** p<0.01, two-way ANOVA with Holm-Sidak multiple comparison test.
Techniques Used: Confocal Microscopy, Immunostaining, Control, MANN-WHITNEY, Comparison, Expressing
Figure Legend Snippet: A: Representative confocal microscopy image of immunostained mitochondrial protein TOMM40 and dsRNA (J2) in control and in patient P3, P4 and P5 fibroblasts. Scale bar: 5µm. B: Quantification of average pixel intensity of immunostaining of dsRNA signal in mitochondria in control cells and in patients’ cells (P3, P4 and P5). Superplot, mean ± SEM; n=3 experiments; each borderless point represents the measure of a cell; each colour is a different experiment; ns indicates non significance, * p<0.05 in one-way ANOVA with Dunnett multiple comparison test test performed on the mean value for each experiment C: Percentage of cells with a J2 signal 1.5-fold above the average of 3 controls. Mean ± SEM; n=3 experiments, each colour is a different experiment. D: Representative confocal microscopy image of immunostained TOMM40 and dsRNA (J2) in control and MTPAP_KO BJ-5ta cells (sg#2) untreated (NT) or treated with actinomycin D (ActD) for up to 24h. Scale bar: 5 µm. E: Quantification of pixel intensity of immunostaining of dsRNA signal in mitochondria in control and MTPAP_KO cells (average of sg#1, #2, #3) untreated (NT) and treated with actinomycin D overtime. Mean ± SEM; n=6 experiments, **** indicates p<0.0001 in two-way ANOVA with Holm-Sidak multiple comparison test. F: Representative confocal microscopy image of immunostained TOMM40 and dsRNA (J2) in MTPAP_KO cells (sg#2) non treated (NT), treated in culture for 10 days with ddC, or untreated in culture but treated after fixation with dsRNA specific RNase III (see Methods). Scale bar: 5 µm. G: Representative confocal microscopy image of immunostained PNPT1 and dsRNA (J2) in control and MTPAP_KO cells (sg#3). Scale bar: 5µm. H-I: Quantification of the median sphericity ( H ) and median volume ( I ) of dsRNA particles in control and MTPAP_KO cells (sg#2). Mean ± SEM; n=3, each dot represents a different cell, each colour represents a different experiment, *** indicates p<0.001, **** p<0.0001 in Mann-Whitney test. J: Schematic representation of the experimental set-up to isolate the cytosolic fraction using digitonin and differential centrifugation. K: Western blot analysis of the different fractions generated to isolate cytosolic fractions. Vinculin is used as a cytosolic marker, Lamin A/C as a nuclear fraction marker, TIM44 and TOM40 as mitochondrial membrane markers and TFAM as mitochondrial matrix marker. Note the absence of all markers but vinculin in the cytosolic fraction.
Techniques Used: Confocal Microscopy, Control, Immunostaining, Comparison, MANN-WHITNEY, Centrifugation, Western Blot, Generated, Marker, Membrane