ti e widefield microscope Search Results


99
Yokogawa Electric csu w1 spinning disk confocal scanner
Csu W1 Spinning Disk Confocal Scanner, supplied by Yokogawa Electric, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/bio_rxiv__2024__11__15__623835-173-14-13?v=Yokogawa+Electric
Average 99 stars, based on 1 article reviews
csu w1 spinning disk confocal scanner - by Bioz Stars, 2026-07
99/100 stars
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99
Nikon tie inverted microscope
Tie Inverted Microscope, supplied by Nikon, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/pmc06546471-535-9-8?v=Nikon
Average 99 stars, based on 1 article reviews
tie inverted microscope - by Bioz Stars, 2026-07
99/100 stars
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90
Hamamatsu orca c13440 flash 4.0 erg [b/w] scmos camera
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Orca C13440 Flash 4.0 Erg [B/W] Scmos Camera, supplied by Hamamatsu, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/pmc09167974-285-10-9?v=Hamamatsu
Average 90 stars, based on 1 article reviews
orca c13440 flash 4.0 erg [b/w] scmos camera - by Bioz Stars, 2026-07
90/100 stars
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99
Nikon widefield nikon eclipse ti e inverted microscope
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Widefield Nikon Eclipse Ti E Inverted Microscope, supplied by Nikon, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/pmc10066036-260-8-9?v=Nikon
Average 99 stars, based on 1 article reviews
widefield nikon eclipse ti e inverted microscope - by Bioz Stars, 2026-07
99/100 stars
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99
Nikon tie inverted widefield fluorescence nikon microscope
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Tie Inverted Widefield Fluorescence Nikon Microscope, supplied by Nikon, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/pmc06084797-882-19-23?v=Nikon
Average 99 stars, based on 1 article reviews
tie inverted widefield fluorescence nikon microscope - by Bioz Stars, 2026-07
99/100 stars
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99
Nikon eclipse ti e c1 plus widefield microscope
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Eclipse Ti E C1 Plus Widefield Microscope, supplied by Nikon, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/pmc11213518-212-15-14?v=Nikon
Average 99 stars, based on 1 article reviews
eclipse ti e c1 plus widefield microscope - by Bioz Stars, 2026-07
99/100 stars
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90
Hamamatsu orca flash 4.0 camera
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Orca Flash 4.0 Camera, supplied by Hamamatsu, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/pm40436920-158-15-14?v=Hamamatsu
Average 90 stars, based on 1 article reviews
orca flash 4.0 camera - by Bioz Stars, 2026-07
90/100 stars
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90
Carl Zeiss zeiss apotome
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Zeiss Apotome, supplied by Carl Zeiss, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/pmc05117151-193-5-5?v=Carl+Zeiss
Average 90 stars, based on 1 article reviews
zeiss apotome - by Bioz Stars, 2026-07
90/100 stars
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96
Nikon eclipse ti e microscope
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Eclipse Ti E Microscope, supplied by Nikon, used in various techniques. Bioz Stars score: 96/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/bio_rxiv__2021__09__30__462547-178-27-26?v=Nikon
Average 96 stars, based on 1 article reviews
eclipse ti e microscope - by Bioz Stars, 2026-07
96/100 stars
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90
Basler microscopy pulse color camera
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Microscopy Pulse Color Camera, supplied by Basler, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/10__1002_slash_sstr__202000074-217-24-23?v=Basler
Average 90 stars, based on 1 article reviews
microscopy pulse color camera - by Bioz Stars, 2026-07
90/100 stars
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99
Yokogawa Electric csu-w1
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Csu W1, supplied by Yokogawa Electric, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/product/ti+e+widefield+microscope/yokogawa+electric___csu_badge?v=Yokogawa+Electric
Average 99 stars, based on 1 article reviews
csu-w1 - by Bioz Stars, 2026-07
99/100 stars
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90
Hamamatsu flash 4.0 v3 scmos
High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca <t>C13440</t> Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="250" height="auto" />
Flash 4.0 V3 Scmos, supplied by Hamamatsu, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca C13440 Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also <xref ref-type=Figure S2 . " width="100%" height="100%">

Journal: iScience

Article Title: MASTL is enriched in cancerous and pluripotent stem cells and influences OCT1/OCT4 levels

doi: 10.1016/j.isci.2022.104459

Figure Lengend Snippet: High MASTL levels correlate with OCT1 and mammosphere formation (A) Western blotting of β3-integrin (ITGB3), OCT1, MASTL, and GAPDH in MDA-MB-231 cells grown as a monolayer (2D) or as mammospheres. (B) Relative protein expression of MASTL to GAPDH, experimental setup shown in (A). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (C) Western blotting of OCT1, MASTL, and GAPDH in MDA-MB-231 cells silenced with siControl or siOCT1 for 48 h. (D) Relative protein expression of MASTL to GAPDH, experimental setup shown in (C), two datapoints collected after 96 h and three after 48 h (n = 5 biologically independent experiments, one sample t-test, mean ± SD). (E) Western blotting of OCT1, MASTL, and tubulin in MDA-MB-231 cells overexpressing EGFP-control (enhanced green fluorescent protein) or hemagglutinin (HA)-tagged OCT1. (F) Relative protein expression of MASTL to tubulin, experimental setup shown in (E). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (G) Representative flow cytometry histograms of MDA-MB-231 cells treated with DMSO control or DCF-DA (2ʹ,7ʹ-Dichlorofluorescin Diacetate) to measure ROS activity after silencing with siControl (gray), siMASTL#6 (red), or siMASTL#7 (orange) for 48 h. (H) Geometric Mean of the DCF-DA signal (ROS activity) in the experimental setup described in (G). (n = 3 biologically independent experiments, unpaired t-test, mean ± SD). (I) Representative images of tetracycline-induced shControl and shMASTL#3 MDA-MB-231 cells grown in mammosphere culture conditions (7 days) and stained with Calcein (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca C13440 Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective). (J) Average mammosphere size (average ferret diameter of spheres in μm) and spheres/1,000 cells plated, experimental setup shown in (I). (n = 3 biologically independent experiments, eight replicate wells/experiment, unpaired t-test, mean ± SEM). (K) Western blotting of OCT1, MASTL, and GAPDH in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (L) Relative protein expression of MASTL to GAPDH, experimental setup shown in (K). (n = 3 biologically independent experiments, one sample t-test, mean ± SD). (M) Representative flow cytometry histograms of CD44 expression in tetracycline-induced (4 days) shControl and shMASTL#3 MDA-MB-231 cells. (N) Geometric mean of CD44 expression in the experimental setup described in (M). (n = 5 biologically independent experiments, unpaired t-test, mean ± SD). See also Figure S2 .

Article Snippet: Images were captured with (Nikon Eclipse Ti-E widefield microscope, Hamamatsu Orca C13440 Flash 4.0 ERG [b/w] sCMOS camera and Plan Apo lambda 20×/0.80, WD 1,000-μm objective).

Techniques: Western Blot, Expressing, Flow Cytometry, Activity Assay, Staining, Microscopy