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nb300 213  (Novus Biologicals)


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    Novus Biologicals nb300 213
    Nb300 213, supplied by Novus Biologicals, used in various techniques. Bioz Stars score: 96/100, based on 159 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/nb300 213/product/Novus Biologicals
    Average 96 stars, based on 159 article reviews
    nb300 213 - by Bioz Stars, 2026-05
    96/100 stars

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    Protein level differences in senescence-associated markers further distinguish neuronal and fibroblast responses to DNA damage (A) Schematic of immunocytochemistry (ICC) performed after IR in healthy dermal fibroblasts and iNs from the same donors (donors: A27, A48, ID98; 3 technical replicates per donor in each condition). 0.2% FBS low serum (LS) treatment was applied to CTL and IR fibroblasts to induce quiescence 72 hours prior to collection. (B) IR iNs and IR fibroblasts were stained for p21 (top left), p16 (top right), LMNB1 (bottom left), and HMGB1 (bottom right). Mean nuclear fluorescence intensity was quantified. (C) Nuclear area of IR iNs and IR fibroblasts quantified by DAPI staining (donors: A27, A48, ID98, 18 technical replicates per donor in each condition). (D) PSD95 staining for IR iNs and IR fibroblasts, imaged by confocal microscopy, and analyzed by Imaris to detect PSD95 spots on <t>MAP2-positive</t> dendrites and normalize to dendrite surface area. Two donors used for PSD95 staining (donors: A27, A48; 3 technical replicates per donor in each condition; donor A48 images and quantification shown in ). Tracks on MAP2 traced in Illustrator. All iNs imaged were quantified with automatic MAP2 tracing to measure p21, p16, LMNB1, HMGB1, and DAPI only in neuronal nuclei or PSD95 only in neuronal dendrites (Supp. Fig. 5). Imaging was performed on the Harmony Operetta CLS system at 63X unless otherwise stated. Nuclear intensity quantification of images performed by the Harmony analysis system and nuclei number after IR provided in Supp. Fig. 4. Statistics were calculated using multiple unpaired t-tests using Welch’s correction with Holm–Šídák adjustment for multiple testing with alpha = 0.05. *p < 0.05, **p < 0.01, ***p < 0.001, ****p < 0.0001, ns: not significant, nd: not detected.
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    Protein level differences in senescence-associated markers further distinguish neuronal and fibroblast responses to DNA damage (A) Schematic of immunocytochemistry (ICC) performed after IR in healthy dermal fibroblasts and iNs from the same donors (donors: A27, A48, ID98; 3 technical replicates per donor in each condition). 0.2% FBS low serum (LS) treatment was applied to CTL and IR fibroblasts to induce quiescence 72 hours prior to collection. (B) IR iNs and IR fibroblasts were stained for p21 (top left), p16 (top right), LMNB1 (bottom left), and HMGB1 (bottom right). Mean nuclear fluorescence intensity was quantified. (C) Nuclear area of IR iNs and IR fibroblasts quantified by DAPI staining (donors: A27, A48, ID98, 18 technical replicates per donor in each condition). (D) PSD95 staining for IR iNs and IR fibroblasts, imaged by confocal microscopy, and analyzed by Imaris to detect PSD95 spots on <t>MAP2-positive</t> dendrites and normalize to dendrite surface area. Two donors used for PSD95 staining (donors: A27, A48; 3 technical replicates per donor in each condition; donor A48 images and quantification shown in ). Tracks on MAP2 traced in Illustrator. All iNs imaged were quantified with automatic MAP2 tracing to measure p21, p16, LMNB1, HMGB1, and DAPI only in neuronal nuclei or PSD95 only in neuronal dendrites (Supp. Fig. 5). Imaging was performed on the Harmony Operetta CLS system at 63X unless otherwise stated. Nuclear intensity quantification of images performed by the Harmony analysis system and nuclei number after IR provided in Supp. Fig. 4. Statistics were calculated using multiple unpaired t-tests using Welch’s correction with Holm–Šídák adjustment for multiple testing with alpha = 0.05. *p < 0.05, **p < 0.01, ***p < 0.001, ****p < 0.0001, ns: not significant, nd: not detected.
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    Protein level differences in senescence-associated markers further distinguish neuronal and fibroblast responses to DNA damage (A) Schematic of immunocytochemistry (ICC) performed after IR in healthy dermal fibroblasts and iNs from the same donors (donors: A27, A48, ID98; 3 technical replicates per donor in each condition). 0.2% FBS low serum (LS) treatment was applied to CTL and IR fibroblasts to induce quiescence 72 hours prior to collection. (B) IR iNs and IR fibroblasts were stained for p21 (top left), p16 (top right), LMNB1 (bottom left), and HMGB1 (bottom right). Mean nuclear fluorescence intensity was quantified. (C) Nuclear area of IR iNs and IR fibroblasts quantified by DAPI staining (donors: A27, A48, ID98, 18 technical replicates per donor in each condition). (D) PSD95 staining for IR iNs and IR fibroblasts, imaged by confocal microscopy, and analyzed by Imaris to detect PSD95 spots on <t>MAP2-positive</t> dendrites and normalize to dendrite surface area. Two donors used for PSD95 staining (donors: A27, A48; 3 technical replicates per donor in each condition; donor A48 images and quantification shown in ). Tracks on MAP2 traced in Illustrator. All iNs imaged were quantified with automatic MAP2 tracing to measure p21, p16, LMNB1, HMGB1, and DAPI only in neuronal nuclei or PSD95 only in neuronal dendrites (Supp. Fig. 5). Imaging was performed on the Harmony Operetta CLS system at 63X unless otherwise stated. Nuclear intensity quantification of images performed by the Harmony analysis system and nuclei number after IR provided in Supp. Fig. 4. Statistics were calculated using multiple unpaired t-tests using Welch’s correction with Holm–Šídák adjustment for multiple testing with alpha = 0.05. *p < 0.05, **p < 0.01, ***p < 0.001, ****p < 0.0001, ns: not significant, nd: not detected.
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    Image Search Results


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    Journal: Redox Biology

    Article Title: Excessive ER-mitochondria coupling: A DRP1-driven mechanism underlying mitochondrial dysfunction and impaired autophagy in stress-induced depression-like behavior in mice

    doi: 10.1016/j.redox.2026.104121

    Figure Lengend Snippet: CSDS upregulates Drp1 expression in hippocampal neurons. A) Differential protein volcano map of CSDS group and Control group (n = 3 samples per group; each sample pooled from 6 hippocampi). Red: significantly upregulated (fold change >1.5); blue: significantly downregulated (fold change >1.5); gray: non-significant. B) CO-IP analysis of Drp1 protein and its ubiquitination level in hippocampus of three groups of mice. One-way ANOVA with Tukey's multiple comparisons test (Treatment, F (2, 15) = 162.8, P < 0.0001; Treatment, F (2, 15) = 12.10, P = 0.0007). Data are expressed as mean ± SEM (n = 6 mice per group). ∗∗ p < 0.01, ∗∗∗ p < 0.001 C) Representative images of Drp1 (green), MAP2 (neuron, red) and DAPI (nucleus, blue) in CA1 of two groups (left) and Pearson correlation coefficient was quantitatively analyzed (right, n = 5 mice brain slices). Scale bar: 50 μm. D) Experimental timeline of viral injection and CSDS modeling; Representative confocal Z-stack 3D reconstructed images of dendritic spines in CA1 (left) and dendritic spines was quantitatively analyzed (right, n = 5 mice brain slices). Scale bar: 2 μm. Student's t -test (P = 0.0041; P = 0.0006). Data are expressed as mean ± SEM. ∗∗ p < 0.01, ∗∗∗ p < 0.001. E) Representative images of Drp1 (green), VGLUT2 (Neuron, red) and DAPI (nucleus, blue) in hippocampal CA1 region of two groups (left) and the percentage of co-localized fluorescence was quantified (right). Scale bar: 50 μm. Two-way ANOVA with Tukey's multiple comparisons test (Interaction, F (2, 24) = 2.671, P = 0.0897). The data were expressed as mean ± SEM (n = 5 mice brain slices). ns, p > 0.05.

    Article Snippet: Multiplex staining was performed using TSA-based immunofluorescence with primary antibodies: Drp1 (CST 12741S, 1:100), MAP2 (ab32454, 1:1000), GFAP (CST 12389, 1:400), IBA1 (ab178846, 1:1000), Vglut1 (CST #27181, 1:800), Vglut2 (ab216463, 1:250), OLIG2 (CST #65915, 1:400), and LAMP1 (CST 99437S, 1:100).

    Techniques: Expressing, Control, Co-Immunoprecipitation Assay, Ubiquitin Proteomics, Injection, Fluorescence

    Protein level differences in senescence-associated markers further distinguish neuronal and fibroblast responses to DNA damage (A) Schematic of immunocytochemistry (ICC) performed after IR in healthy dermal fibroblasts and iNs from the same donors (donors: A27, A48, ID98; 3 technical replicates per donor in each condition). 0.2% FBS low serum (LS) treatment was applied to CTL and IR fibroblasts to induce quiescence 72 hours prior to collection. (B) IR iNs and IR fibroblasts were stained for p21 (top left), p16 (top right), LMNB1 (bottom left), and HMGB1 (bottom right). Mean nuclear fluorescence intensity was quantified. (C) Nuclear area of IR iNs and IR fibroblasts quantified by DAPI staining (donors: A27, A48, ID98, 18 technical replicates per donor in each condition). (D) PSD95 staining for IR iNs and IR fibroblasts, imaged by confocal microscopy, and analyzed by Imaris to detect PSD95 spots on MAP2-positive dendrites and normalize to dendrite surface area. Two donors used for PSD95 staining (donors: A27, A48; 3 technical replicates per donor in each condition; donor A48 images and quantification shown in ). Tracks on MAP2 traced in Illustrator. All iNs imaged were quantified with automatic MAP2 tracing to measure p21, p16, LMNB1, HMGB1, and DAPI only in neuronal nuclei or PSD95 only in neuronal dendrites (Supp. Fig. 5). Imaging was performed on the Harmony Operetta CLS system at 63X unless otherwise stated. Nuclear intensity quantification of images performed by the Harmony analysis system and nuclei number after IR provided in Supp. Fig. 4. Statistics were calculated using multiple unpaired t-tests using Welch’s correction with Holm–Šídák adjustment for multiple testing with alpha = 0.05. *p < 0.05, **p < 0.01, ***p < 0.001, ****p < 0.0001, ns: not significant, nd: not detected.

    Journal: bioRxiv

    Article Title: DNA damage drives a unique, Alzheimer’s disease-relevant senescent state in neurons

    doi: 10.64898/2026.04.02.716205

    Figure Lengend Snippet: Protein level differences in senescence-associated markers further distinguish neuronal and fibroblast responses to DNA damage (A) Schematic of immunocytochemistry (ICC) performed after IR in healthy dermal fibroblasts and iNs from the same donors (donors: A27, A48, ID98; 3 technical replicates per donor in each condition). 0.2% FBS low serum (LS) treatment was applied to CTL and IR fibroblasts to induce quiescence 72 hours prior to collection. (B) IR iNs and IR fibroblasts were stained for p21 (top left), p16 (top right), LMNB1 (bottom left), and HMGB1 (bottom right). Mean nuclear fluorescence intensity was quantified. (C) Nuclear area of IR iNs and IR fibroblasts quantified by DAPI staining (donors: A27, A48, ID98, 18 technical replicates per donor in each condition). (D) PSD95 staining for IR iNs and IR fibroblasts, imaged by confocal microscopy, and analyzed by Imaris to detect PSD95 spots on MAP2-positive dendrites and normalize to dendrite surface area. Two donors used for PSD95 staining (donors: A27, A48; 3 technical replicates per donor in each condition; donor A48 images and quantification shown in ). Tracks on MAP2 traced in Illustrator. All iNs imaged were quantified with automatic MAP2 tracing to measure p21, p16, LMNB1, HMGB1, and DAPI only in neuronal nuclei or PSD95 only in neuronal dendrites (Supp. Fig. 5). Imaging was performed on the Harmony Operetta CLS system at 63X unless otherwise stated. Nuclear intensity quantification of images performed by the Harmony analysis system and nuclei number after IR provided in Supp. Fig. 4. Statistics were calculated using multiple unpaired t-tests using Welch’s correction with Holm–Šídák adjustment for multiple testing with alpha = 0.05. *p < 0.05, **p < 0.01, ***p < 0.001, ****p < 0.0001, ns: not significant, nd: not detected.

    Article Snippet: Cells were then incubated with primary antibodies at 4°C overnight (γH2AX, abcam, ab81299, 1:250; 1:1000; pATM, Life Technologies, MA1-2020, 1:250; p21, abcam, ab109520, 1:100; p16, abcam, ab270058, 1:50; LMNB1, abcam, ab229025, 1:1000; HMGB1, abcam, ab79823, 1:250; 53BP1, abcam, ab175933, 1:200, PSD95, Life Technologies, MA1-046, 1:300; MAP2, Novus Biologicals, NB300-213, 1:400).

    Techniques: Immunocytochemistry, Staining, Fluorescence, Confocal Microscopy, Imaging

    DNA damage induces greater damage lesions and a slower DNA repair-associated response in neurons compared to fibroblasts (A) Schematic of immunocytochemistry (ICC) performed over time after IR in healthy dermal fibroblasts and iNs from the same donors (donors: A48, ID97; 3 technical replicates per donor in each condition). (B-D) iNs and fibroblasts were stained for 53BP1 (B), γH2AX (C), and pATM (D) at 0 min, 15 min, 2h, and 24h after IR with magnified images from the viewfield in the bottom right of each image. Relative fold change (right panels) was calculated from mean foci number per nucleus (middle panels). All iNs imaged were quantified with automatic MAP2 tracing to measure 53BP1, γH2AX, and pATM foci only in neuronal nuclei (Supp. Fig. 5). Imaging was performed on the Harmony Operetta CLS system at 63X. Foci quantification of images performed by the Harmony analysis system. Intensity over time without relative fold change calculations provided in Supp. Fig. 6 along with nuclei number over time after IR. Statistics were calculated by two-way ANOVA (or Mixed Model) and corrected for multiple comparisons using the Dunnett method and reporting multiplicity-adjusted p-value for each comparison with alpha = 0.05. *p < 0.05, **p < 0.01, ***p < 0.001, ****p < 0.0001, ns: not significant, nd: not detected.

    Journal: bioRxiv

    Article Title: DNA damage drives a unique, Alzheimer’s disease-relevant senescent state in neurons

    doi: 10.64898/2026.04.02.716205

    Figure Lengend Snippet: DNA damage induces greater damage lesions and a slower DNA repair-associated response in neurons compared to fibroblasts (A) Schematic of immunocytochemistry (ICC) performed over time after IR in healthy dermal fibroblasts and iNs from the same donors (donors: A48, ID97; 3 technical replicates per donor in each condition). (B-D) iNs and fibroblasts were stained for 53BP1 (B), γH2AX (C), and pATM (D) at 0 min, 15 min, 2h, and 24h after IR with magnified images from the viewfield in the bottom right of each image. Relative fold change (right panels) was calculated from mean foci number per nucleus (middle panels). All iNs imaged were quantified with automatic MAP2 tracing to measure 53BP1, γH2AX, and pATM foci only in neuronal nuclei (Supp. Fig. 5). Imaging was performed on the Harmony Operetta CLS system at 63X. Foci quantification of images performed by the Harmony analysis system. Intensity over time without relative fold change calculations provided in Supp. Fig. 6 along with nuclei number over time after IR. Statistics were calculated by two-way ANOVA (or Mixed Model) and corrected for multiple comparisons using the Dunnett method and reporting multiplicity-adjusted p-value for each comparison with alpha = 0.05. *p < 0.05, **p < 0.01, ***p < 0.001, ****p < 0.0001, ns: not significant, nd: not detected.

    Article Snippet: Cells were then incubated with primary antibodies at 4°C overnight (γH2AX, abcam, ab81299, 1:250; 1:1000; pATM, Life Technologies, MA1-2020, 1:250; p21, abcam, ab109520, 1:100; p16, abcam, ab270058, 1:50; LMNB1, abcam, ab229025, 1:1000; HMGB1, abcam, ab79823, 1:250; 53BP1, abcam, ab175933, 1:200, PSD95, Life Technologies, MA1-046, 1:300; MAP2, Novus Biologicals, NB300-213, 1:400).

    Techniques: Immunocytochemistry, Staining, Imaging, Comparison