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R&D Systems il 6 elisa kit

(a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐originated lymph vessels. (b) Effects of water intake on changes in the concentration of IL‐1β in the lymph. (c) Effects of water intake on changes in the concentration <t>of</t> <t>IL‐6</t> in the lymph. (d) Effects of water intake on changes in the concentration of IL‐10 in the lymph. The open column, control; the black column, water intake. The error bars represent SDs.

Il 6 Elisa Kit, supplied by R&D Systems, used in various techniques. Bioz Stars score: 96/100, based on 1208 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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1) Product Images from "Water intake regulates mucosal immunity in rat jejunal villi via IL ‐1β, IL ‐6, and IL ‐10"

Article Title: Water intake regulates mucosal immunity in rat jejunal villi via IL ‐1β, IL ‐6, and IL ‐10

Journal: Physiological Reports

doi: 10.14814/phy2.70891

Figure Legend Snippet: (a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐originated lymph vessels. (b) Effects of water intake on changes in the concentration of IL‐1β in the lymph. (c) Effects of water intake on changes in the concentration of IL‐6 in the lymph. (d) Effects of water intake on changes in the concentration of IL‐10 in the lymph. The open column, control; the black column, water intake. The error bars represent SDs.

Techniques Used: Concentration Assay, Control

(a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐derived lymph vessels in the absence (white column) and presence of clodronate (oblique line column). (b) Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐1β in the lymph. Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐6 in the lymph. Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐10 in the lymph. The error bars represent SDs.

Figure Legend Snippet: (a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐derived lymph vessels in the absence (white column) and presence of clodronate (oblique line column). (b) Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐1β in the lymph. Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐6 in the lymph. Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐10 in the lymph. The error bars represent SDs.

Techniques Used: Derivative Assay, Concentration Assay

Figure Legend Snippet: (a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐derived lymph vessels in the absence (white column) and presence of a MyD88 inhibitor (oblique line column). (b) Effects of water intake without (white column) and with a MyD88 inhibitor (oblique line column) on changes in the concentration of IL‐1β in the lymph. (c) Effects of water intake without (white column) and with a MyD88 inhibitor (oblique line column) on changes in the concentration of IL‐6 in the lymph. (d) Effects of water intake without (white column) and with a MyD88 inhibitor (oblique line column) on changes in the concentration of IL‐10 in the lymph. The error bars represent the SDs.

Techniques Used: Derivative Assay, Concentration Assay

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Image Search Results

Journal: Physiological Reports

Article Title: Water intake regulates mucosal immunity in rat jejunal villi via IL ‐1β, IL ‐6, and IL ‐10

doi: 10.14814/phy2.70891

Figure Lengend Snippet: (a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐originated lymph vessels. (b) Effects of water intake on changes in the concentration of IL‐1β in the lymph. (c) Effects of water intake on changes in the concentration of IL‐6 in the lymph. (d) Effects of water intake on changes in the concentration of IL‐10 in the lymph. The open column, control; the black column, water intake. The error bars represent SDs.

Article Snippet: The concentrations of cytokines in the lymph were measured using enzyme‐linked immunosorbent assay (ELISA) kits: a rat IL‐1β ELISA quantitative kit (catalog no. RLB00; R&D Systems, Minneapolis, MN, USA), an IL‐6 ELISA kit (catalog no. R6000B; R&D Systems, Minneapolis, MN, USA), and a mouse/rat IL‐10 ELISA kit (catalog no. KE20003; Rosemont, IL, USA) (Arai et al., ).

Techniques: Concentration Assay, Control

Journal: Physiological Reports

Article Title: Water intake regulates mucosal immunity in rat jejunal villi via IL ‐1β, IL ‐6, and IL ‐10

doi: 10.14814/phy2.70891

Figure Lengend Snippet: (a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐derived lymph vessels in the absence (white column) and presence of clodronate (oblique line column). (b) Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐1β in the lymph. Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐6 in the lymph. Effects of water intake without (white column) and with clodronate (oblique line column) on changes in the concentration of IL‐10 in the lymph. The error bars represent SDs.

Techniques: Derivative Assay, Concentration Assay

Journal: Physiological Reports

Article Title: Water intake regulates mucosal immunity in rat jejunal villi via IL ‐1β, IL ‐6, and IL ‐10

doi: 10.14814/phy2.70891

Figure Lengend Snippet: (a) Effects of water intake on changes in lymph volume collected over set intervals of 60 min in rat jejunum‐derived lymph vessels in the absence (white column) and presence of a MyD88 inhibitor (oblique line column). (b) Effects of water intake without (white column) and with a MyD88 inhibitor (oblique line column) on changes in the concentration of IL‐1β in the lymph. (c) Effects of water intake without (white column) and with a MyD88 inhibitor (oblique line column) on changes in the concentration of IL‐6 in the lymph. (d) Effects of water intake without (white column) and with a MyD88 inhibitor (oblique line column) on changes in the concentration of IL‐10 in the lymph. The error bars represent the SDs.

Techniques: Derivative Assay, Concentration Assay

Journal: Journal of Inflammation Research

Article Title: Acupuncture Activates PI3K/Akt Pathway to Promote Spinal Microglial M2 Polarization and Alleviate Spastic Hemiplegia Following Ischemic Stroke

doi: 10.2147/JIR.S592917

Figure Lengend Snippet: Acupuncture shifted spinal microglia toward the M2 phenotype, modified spinal inflammation milieu, restored the E/I balancing in the spinal motor circuit and activated the spinal PI3K/Akt pathway in MCAO rats with spastic hemiplegia. Immunofluorescence of microglial polarization state: representative images of CD32 (M1 marker, green) and Iba-1 (microglial marker, red) co-localization by immunofluorescence ( A ); representative images of CD206 (M2 marker, green) and Iba-1 (red) co-localization by immunofluorescence ( B ) with all nuclei of cells stained by DAPI (blue); scale bar, 50 μm; the semi-quantitative fluorescent intensity results of CD32 ( C ) and CD206 ( D ). Immunofluorescence of synaptic boutons in motor circuit: representative images of vGluT1 immunoreactive boutons (marking the proprioceptive terminals, red) on CTB-labeled motor neurons (MNs, green) ( E ); representative images of vGluT1 boutons (red) contacting vGAT immunoreactive boutons (marking GABAergic synapses, green) ( F ); scale bar, 10 μm, 2 μm; fold change of vGluT1 boutons on MNs ( G ); ratio of vGluT1 boutons opposed by vGAT boutons ( H ). Representative Western blot bands ( I ) and quantitative results for CD32 ( J ), CD206 ( K ), vGluT1 ( L ), vGAT ( M ), p-PI3K/PI3K ( N ), and p-Akt/Akt ( O ) protein expressions relative to GAPDH protein. The mRNA levels of CD32 ( P ) and CD206 ( Q ) were detected by RT-qPCR. The concentrations of TNF-α ( R ), IL-6 ( S ), TGF-β ( T ), IL-10 ( U ), Glu ( V ), GABA ( W ) were detected by ELISA. N = 6 per group. Data were expressed as mean ± SD. **P<0.01,***P<0.001 versus M+AP group; ### P<0.001 versus M group.

Article Snippet: The levels of TNF-α (EK0526, Boster Biological), IL-6 (EK0412, Boster Biological), and TGF-β (EK0514, Boster Biological), IL-10 (EK0418, Boster Biological) were determined to assess neuroinflammation.

Techniques: Modification, Immunofluorescence, Marker, Staining, Labeling, Western Blot, Quantitative RT-PCR, Enzyme-linked Immunosorbent Assay

Inhibition of M1 polarization of microglia mitigated spinal inflammatory milieu and facilitated the restoration of spinal E/I balance in MCAO rats with spastic hemiplegia. Immunofluorescence of microglial polarization state: representative images of CD32 (green) and Iba-1 (red) co-localization by immunofluorescence ( A ) representative images of CD206 (green) and Iba-1 (red) co-localization by immunofluorescence ( B ) with all nuclei of cells stained by DAPI (blue); scale bar, 50 μm; the semi-quantitative fluorescent intensity results of CD32 ( C ) and CD206 ( D ). Immunofluorescence of synaptic boutons in motor circuit: representative images of vGluT1 immunoreactive boutons (red) on CTB-labeled MNs (green) ( E ) representative images of vGluT1 boutons (red) contacting vGAT immunoreactive boutons (green) ( F ) scale bar, 10 μm, 2 μm; fold change of vGluT1 boutons on MNs ( G ) ratio of vGluT1 boutons opposed by vGAT boutons ( H ). Representative Western blot bands ( I ) and quantitative results for CD32 ( J ) CD206 ( K ) vGluT1 ( L ) vGAT ( M ) protein expression relative to GAPDH protein. The mRNA levels of CD32 ( N ) and CD206 ( O ) were detected by RT-qPCR. The concentrations of TNF-α ( P ) IL-6 ( Q ) TGF-β ( R ) IL-10 ( S ) Glu ( T ) GABA ( U ) were detected by ELISA. N = 6 per group. Data were expressed as mean ± SD. **P<0.01, ***P<0.001 versus M+MC group; ### P<0.001 versus M group.

Journal: Journal of Inflammation Research

Article Title: Acupuncture Activates PI3K/Akt Pathway to Promote Spinal Microglial M2 Polarization and Alleviate Spastic Hemiplegia Following Ischemic Stroke

doi: 10.2147/JIR.S592917

Figure Lengend Snippet: Inhibition of M1 polarization of microglia mitigated spinal inflammatory milieu and facilitated the restoration of spinal E/I balance in MCAO rats with spastic hemiplegia. Immunofluorescence of microglial polarization state: representative images of CD32 (green) and Iba-1 (red) co-localization by immunofluorescence ( A ) representative images of CD206 (green) and Iba-1 (red) co-localization by immunofluorescence ( B ) with all nuclei of cells stained by DAPI (blue); scale bar, 50 μm; the semi-quantitative fluorescent intensity results of CD32 ( C ) and CD206 ( D ). Immunofluorescence of synaptic boutons in motor circuit: representative images of vGluT1 immunoreactive boutons (red) on CTB-labeled MNs (green) ( E ) representative images of vGluT1 boutons (red) contacting vGAT immunoreactive boutons (green) ( F ) scale bar, 10 μm, 2 μm; fold change of vGluT1 boutons on MNs ( G ) ratio of vGluT1 boutons opposed by vGAT boutons ( H ). Representative Western blot bands ( I ) and quantitative results for CD32 ( J ) CD206 ( K ) vGluT1 ( L ) vGAT ( M ) protein expression relative to GAPDH protein. The mRNA levels of CD32 ( N ) and CD206 ( O ) were detected by RT-qPCR. The concentrations of TNF-α ( P ) IL-6 ( Q ) TGF-β ( R ) IL-10 ( S ) Glu ( T ) GABA ( U ) were detected by ELISA. N = 6 per group. Data were expressed as mean ± SD. **P<0.01, ***P<0.001 versus M+MC group; ### P<0.001 versus M group.

Techniques: Inhibition, Immunofluorescence, Staining, Labeling, Western Blot, Expressing, Quantitative RT-PCR, Enzyme-linked Immunosorbent Assay

Acupuncture mitigated excitability of spinal motor circuits and inflammatory milieu via PI3K/Akt pathway in MCAO rats with spastic hemiplegia. Immunofluorescence of synaptic boutons in motor circuit: representative images of vGluT1 immunoreactive boutons (red) on CTB-labeled MNs (green) ( A ); representative images of vGluT1 boutons (red) contacting vGAT immunoreactive boutons (green) ( B ); scale bar, 10 μm, 2 μm; fold change of vGluT1 boutons on MNs ( C ); ratio of vGluT1 boutons opposed by vGAT boutons ( D ). Representative Western blot bands ( E ) and quantitative results for CD32 ( F ) CD206 ( G ) vGluT1 ( H ) vGAT ( I ) protein expression relative to GAPDH protein. The mRNA levels of CD32 ( J ) and CD206 ( K ) were detected by RT-qPCR. The concentrations of TNF-α ( L ) IL-6 ( M ) TGF-β ( N ) IL-10 ( O ) Glu ( P ) GABA ( Q ) were detected by ELISA. N = 6 per group. Data were expressed as mean ± SD. ***P<0.001 versus M+AP+Veh group; ## P<0.01, ### P<0.001 versus M+Veh group.

Journal: Journal of Inflammation Research

Article Title: Acupuncture Activates PI3K/Akt Pathway to Promote Spinal Microglial M2 Polarization and Alleviate Spastic Hemiplegia Following Ischemic Stroke

doi: 10.2147/JIR.S592917

Figure Lengend Snippet: Acupuncture mitigated excitability of spinal motor circuits and inflammatory milieu via PI3K/Akt pathway in MCAO rats with spastic hemiplegia. Immunofluorescence of synaptic boutons in motor circuit: representative images of vGluT1 immunoreactive boutons (red) on CTB-labeled MNs (green) ( A ); representative images of vGluT1 boutons (red) contacting vGAT immunoreactive boutons (green) ( B ); scale bar, 10 μm, 2 μm; fold change of vGluT1 boutons on MNs ( C ); ratio of vGluT1 boutons opposed by vGAT boutons ( D ). Representative Western blot bands ( E ) and quantitative results for CD32 ( F ) CD206 ( G ) vGluT1 ( H ) vGAT ( I ) protein expression relative to GAPDH protein. The mRNA levels of CD32 ( J ) and CD206 ( K ) were detected by RT-qPCR. The concentrations of TNF-α ( L ) IL-6 ( M ) TGF-β ( N ) IL-10 ( O ) Glu ( P ) GABA ( Q ) were detected by ELISA. N = 6 per group. Data were expressed as mean ± SD. ***P<0.001 versus M+AP+Veh group; ## P<0.01, ### P<0.001 versus M+Veh group.

Techniques: Immunofluorescence, Labeling, Western Blot, Expressing, Quantitative RT-PCR, Enzyme-linked Immunosorbent Assay

Journal: iScience

Article Title: A pharmacological rat model of recurrent pelvic pain exhibiting hyperalgesia and depression-like behaviors

doi: 10.1016/j.isci.2026.115059

Figure Lengend Snippet: Prostaglandin dysregulation and inflammatory response in the RPP model (A–C) Uterine PGF 2α (A), PGE 2 (B), and PGF 2α /PGE 2 ratio (C) on days 12 and 24 of RPP modeling ( n = 3). (D) The protein levels of COX-2 in the uterine tissue on days 12 and 24 of RPP modeling ( n = 3). (E–G) The levels of IL-1β (E), IL-6 (F), and TNF-α (G) in the serum on days 12 and 24 of RPP modeling ( n = 3). Data are presented as the mean ± SD; ∗ p < 0.05, ∗∗ p < 0.01, ∗∗∗ p < 0.001, one-way ANOVA.

Article Snippet: Rat IL-6 ELISA Kit , Elabscience , Cat# E-EL-R0015.

Techniques:

ATF6 plays a protective role in renal ischemia-reperfusion injury (A–B) The levels of serum Cr and BUN in mice. (C–D) The levels of serum IL-6 and TNF-α in mice. (E–F) The representative images and kidney injury assessment score of HE staining of the kidney. Ceapin-A7 (10 μM) is an ATF6 inhibitor, and AA147 (10 μM) is an ATF6 agonist. Data represent mean ± SDs, and statistical analysis was performed using one-way ANOVA. (∗ p < 0.05).

Journal: iScience

Article Title: ATF6 ameliorates renal warm ischemia-reperfusion injury through FHL2-mediated NF-κB signaling pathway

doi: 10.1016/j.isci.2026.115173

Figure Lengend Snippet: ATF6 plays a protective role in renal ischemia-reperfusion injury (A–B) The levels of serum Cr and BUN in mice. (C–D) The levels of serum IL-6 and TNF-α in mice. (E–F) The representative images and kidney injury assessment score of HE staining of the kidney. Ceapin-A7 (10 μM) is an ATF6 inhibitor, and AA147 (10 μM) is an ATF6 agonist. Data represent mean ± SDs, and statistical analysis was performed using one-way ANOVA. (∗ p < 0.05).

Article Snippet: IL-6 ELISA kit , Boster , EK0412.

Techniques: Staining

Journal: iScience

Article Title: ATF6 ameliorates renal warm ischemia-reperfusion injury through FHL2-mediated NF-κB signaling pathway

doi: 10.1016/j.isci.2026.115173

Figure Lengend Snippet: ATF6 plays a protective role in renal ischemia-reperfusion injury (A–B) The levels of serum Cr and BUN in mice. (C–D) The levels of serum IL-6 and TNF-α in mice. (E–F) The representative images and kidney injury assessment score of HE staining of the kidney. (G–H) RT-qPCR analysis of TNF-α and IL-6 expression in cultured HK-2 in response to H/R treatment. (I–J) RT-qPCR analysis of IL-6 and TNF-α expression in cultured HK-2 in response to H/R using siATF6. Data represent mean ± SDs, and statistical analysis was performed using one-way ANOVA. (∗ p < 0.05).

Article Snippet: IL-6 ELISA kit , Boster , EK0412.

Techniques: Staining, Quantitative RT-PCR, Expressing, Cell Culture