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recombinant mouse npnt rmnpnt  (R&D Systems)


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    R&D Systems recombinant mouse npnt rmnpnt
    Cell surface distribution of <t>NPNT</t> in 66cl4 cells. (A) Immunofluorescence microscopy showing extracellular NPNT detected on 66cl4 cells expressing wild‐type NPNT and 66cl4‐ EV cells when preincubated with rm NPNT for 1 h prior fixing. 66cl4‐ EV was used as a negative control. Detection of collagen V on 66cl4‐ NPNT cells was used as a positive control. Primary antibodies were visualized with Alexa Fluor 488. Nucleus is stained blue with Hoechst. Scale bar 10 μm. (B) Z profile comparing the green and blue channels was calculated by normalizing mean intensity per slice in the stack for each channel using the image of 66cl4 cells overexpressing NPNT shown above. (C) Brightfield microscopy images of 66cl4‐ EV cells growing on uncoated plates ( EV ) in contrast to rm NPNT ‐coated plates ( EV rm NPNT ) at 24 h.
    Recombinant Mouse Npnt Rmnpnt, supplied by R&D Systems, used in various techniques. Bioz Stars score: 93/100, based on 13 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/recombinant mouse npnt rmnpnt/product/R&D Systems
    Average 93 stars, based on 13 article reviews
    recombinant mouse npnt rmnpnt - by Bioz Stars, 2026-03
    93/100 stars

    Images

    1) Product Images from "Nephronectin mediates p38 MAPK ‐induced cell viability via its integrin‐binding enhancer motif"

    Article Title: Nephronectin mediates p38 MAPK ‐induced cell viability via its integrin‐binding enhancer motif

    Journal: FEBS Open Bio

    doi: 10.1002/2211-5463.12544

    Cell surface distribution of NPNT in 66cl4 cells. (A) Immunofluorescence microscopy showing extracellular NPNT detected on 66cl4 cells expressing wild‐type NPNT and 66cl4‐ EV cells when preincubated with rm NPNT for 1 h prior fixing. 66cl4‐ EV was used as a negative control. Detection of collagen V on 66cl4‐ NPNT cells was used as a positive control. Primary antibodies were visualized with Alexa Fluor 488. Nucleus is stained blue with Hoechst. Scale bar 10 μm. (B) Z profile comparing the green and blue channels was calculated by normalizing mean intensity per slice in the stack for each channel using the image of 66cl4 cells overexpressing NPNT shown above. (C) Brightfield microscopy images of 66cl4‐ EV cells growing on uncoated plates ( EV ) in contrast to rm NPNT ‐coated plates ( EV rm NPNT ) at 24 h.
    Figure Legend Snippet: Cell surface distribution of NPNT in 66cl4 cells. (A) Immunofluorescence microscopy showing extracellular NPNT detected on 66cl4 cells expressing wild‐type NPNT and 66cl4‐ EV cells when preincubated with rm NPNT for 1 h prior fixing. 66cl4‐ EV was used as a negative control. Detection of collagen V on 66cl4‐ NPNT cells was used as a positive control. Primary antibodies were visualized with Alexa Fluor 488. Nucleus is stained blue with Hoechst. Scale bar 10 μm. (B) Z profile comparing the green and blue channels was calculated by normalizing mean intensity per slice in the stack for each channel using the image of 66cl4 cells overexpressing NPNT shown above. (C) Brightfield microscopy images of 66cl4‐ EV cells growing on uncoated plates ( EV ) in contrast to rm NPNT ‐coated plates ( EV rm NPNT ) at 24 h.

    Techniques Used: Immunofluorescence, Microscopy, Expressing, Negative Control, Positive Control, Staining

    Reverse‐phase protein array analysis of NPNT ‐mediated signaling. The Venn diagram includes number of proteins significantly regulated and/or modified ( P < 0. 05) in all four biological replicates. (A) The pink circle in the Venn diagram, ‘ NPNT vs EV ’, denotes the log‐fold change values triggered in 66cl4‐ NPNT cells in comparison with 66cl4‐ EV cells. The blue circle, ‘ EV rm NPNT vs EV ’, represents 66cl4‐ EV cells cultured on rm NPNT ( EV rm NPNT ) in comparison with 66cl4‐ EV cells seeded in noncoated wells. The purple circle represents proteins regulated by the integrin‐binding motifs of NPNT ; the effect of a single mutation in the RGD motif ( RGD → RGE ) versus mutations in both RGD and EIE motifs ( RGD ‐ EIE ‐> RGE ‐ AIA ). (B) Box plot showing log2 protein abundance of the four overlapping proteins from the Venn diagram.
    Figure Legend Snippet: Reverse‐phase protein array analysis of NPNT ‐mediated signaling. The Venn diagram includes number of proteins significantly regulated and/or modified ( P < 0. 05) in all four biological replicates. (A) The pink circle in the Venn diagram, ‘ NPNT vs EV ’, denotes the log‐fold change values triggered in 66cl4‐ NPNT cells in comparison with 66cl4‐ EV cells. The blue circle, ‘ EV rm NPNT vs EV ’, represents 66cl4‐ EV cells cultured on rm NPNT ( EV rm NPNT ) in comparison with 66cl4‐ EV cells seeded in noncoated wells. The purple circle represents proteins regulated by the integrin‐binding motifs of NPNT ; the effect of a single mutation in the RGD motif ( RGD → RGE ) versus mutations in both RGD and EIE motifs ( RGD ‐ EIE ‐> RGE ‐ AIA ). (B) Box plot showing log2 protein abundance of the four overlapping proteins from the Venn diagram.

    Techniques Used: Protein Array, Modification, Comparison, Cell Culture, Binding Assay, Mutagenesis, Quantitative Proteomics

    Top predicted molecular and cellular functions. RPPA results from RGE vs RGE‐AIA group were analyzed using the web‐based software application ingenuity pathway analysis (IPA) tool to identify the most significant NPNT‐responsive functions
    Figure Legend Snippet: Top predicted molecular and cellular functions. RPPA results from RGE vs RGE‐AIA group were analyzed using the web‐based software application ingenuity pathway analysis (IPA) tool to identify the most significant NPNT‐responsive functions

    Techniques Used: Software, Activation Assay

    Nephronectin mediates cell viability via p38 signaling pathways. (A) Indicated variants of 66cl4 cells were treated with (±) 4 μ m p38 MAPK inhibitor ( BIRB 796) for 24 h, in addition to serum deprivation. Where indicated, 66cl4‐ EV cells were stimulated by adding 2 μg·mL −1 rm NPNT to the cell culture medium. Cell viability was determined using CellTiter‐Glo. (B) Viability of NPNT expressing, 4T1 cells with a NPNT ‐targeted short hairpin (sh‐ NPNT ) and a nontargeting sh RNA (sh‐ctr) was tested using CellTiter‐Glo. Significance is tested using a two‐tailed Student's t‐test. * P < 0. 05, ** P < 0. 005, *** P < 0. 0001. Error bars represent SD . N = number of independent experiments, n = total number of replicates in each test group. (C) Illustration summarizing the cellular effects of integrin binding to wild‐type or mutated NPNT via p38 MAPK .
    Figure Legend Snippet: Nephronectin mediates cell viability via p38 signaling pathways. (A) Indicated variants of 66cl4 cells were treated with (±) 4 μ m p38 MAPK inhibitor ( BIRB 796) for 24 h, in addition to serum deprivation. Where indicated, 66cl4‐ EV cells were stimulated by adding 2 μg·mL −1 rm NPNT to the cell culture medium. Cell viability was determined using CellTiter‐Glo. (B) Viability of NPNT expressing, 4T1 cells with a NPNT ‐targeted short hairpin (sh‐ NPNT ) and a nontargeting sh RNA (sh‐ctr) was tested using CellTiter‐Glo. Significance is tested using a two‐tailed Student's t‐test. * P < 0. 05, ** P < 0. 005, *** P < 0. 0001. Error bars represent SD . N = number of independent experiments, n = total number of replicates in each test group. (C) Illustration summarizing the cellular effects of integrin binding to wild‐type or mutated NPNT via p38 MAPK .

    Techniques Used: Protein-Protein interactions, Cell Culture, Expressing, Two Tailed Test, Binding Assay



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    recombinant mouse npnt rmnpnt  (R&D Systems)
    93
    R&D Systems recombinant mouse npnt rmnpnt
    Cell surface distribution of <t>NPNT</t> in 66cl4 cells. (A) Immunofluorescence microscopy showing extracellular NPNT detected on 66cl4 cells expressing wild‐type NPNT and 66cl4‐ EV cells when preincubated with rm NPNT for 1 h prior fixing. 66cl4‐ EV was used as a negative control. Detection of collagen V on 66cl4‐ NPNT cells was used as a positive control. Primary antibodies were visualized with Alexa Fluor 488. Nucleus is stained blue with Hoechst. Scale bar 10 μm. (B) Z profile comparing the green and blue channels was calculated by normalizing mean intensity per slice in the stack for each channel using the image of 66cl4 cells overexpressing NPNT shown above. (C) Brightfield microscopy images of 66cl4‐ EV cells growing on uncoated plates ( EV ) in contrast to rm NPNT ‐coated plates ( EV rm NPNT ) at 24 h.
    Recombinant Mouse Npnt Rmnpnt, supplied by R&D Systems, used in various techniques. Bioz Stars score: 93/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
    https://www.bioz.com/result/recombinant mouse npnt rmnpnt/product/R&D Systems
    Average 93 stars, based on 1 article reviews
    recombinant mouse npnt rmnpnt - by Bioz Stars, 2026-03
    93/100 stars
    		  Buy from Supplier

    Image Search Results


    Cell surface distribution of NPNT in 66cl4 cells. (A) Immunofluorescence microscopy showing extracellular NPNT detected on 66cl4 cells expressing wild‐type NPNT and 66cl4‐ EV cells when preincubated with rm NPNT for 1 h prior fixing. 66cl4‐ EV was used as a negative control. Detection of collagen V on 66cl4‐ NPNT cells was used as a positive control. Primary antibodies were visualized with Alexa Fluor 488. Nucleus is stained blue with Hoechst. Scale bar 10 μm. (B) Z profile comparing the green and blue channels was calculated by normalizing mean intensity per slice in the stack for each channel using the image of 66cl4 cells overexpressing NPNT shown above. (C) Brightfield microscopy images of 66cl4‐ EV cells growing on uncoated plates ( EV ) in contrast to rm NPNT ‐coated plates ( EV rm NPNT ) at 24 h.

    Journal: FEBS Open Bio

    Article Title: Nephronectin mediates p38 MAPK ‐induced cell viability via its integrin‐binding enhancer motif

    doi: 10.1002/2211-5463.12544

    Figure Lengend Snippet: Cell surface distribution of NPNT in 66cl4 cells. (A) Immunofluorescence microscopy showing extracellular NPNT detected on 66cl4 cells expressing wild‐type NPNT and 66cl4‐ EV cells when preincubated with rm NPNT for 1 h prior fixing. 66cl4‐ EV was used as a negative control. Detection of collagen V on 66cl4‐ NPNT cells was used as a positive control. Primary antibodies were visualized with Alexa Fluor 488. Nucleus is stained blue with Hoechst. Scale bar 10 μm. (B) Z profile comparing the green and blue channels was calculated by normalizing mean intensity per slice in the stack for each channel using the image of 66cl4 cells overexpressing NPNT shown above. (C) Brightfield microscopy images of 66cl4‐ EV cells growing on uncoated plates ( EV ) in contrast to rm NPNT ‐coated plates ( EV rm NPNT ) at 24 h.

    Article Snippet: The effect of incubating 66cl4‐EV cells with 2 μg·mL −1 recombinant mouse NPNT (rmNPNT) (R&D systems, Minneapolis, MN, USA; Cat: 4298‐NP‐050) in PBS for 1 h prior fixing was also investigated.

    Techniques: Immunofluorescence, Microscopy, Expressing, Negative Control, Positive Control, Staining

    Reverse‐phase protein array analysis of NPNT ‐mediated signaling. The Venn diagram includes number of proteins significantly regulated and/or modified ( P < 0. 05) in all four biological replicates. (A) The pink circle in the Venn diagram, ‘ NPNT vs EV ’, denotes the log‐fold change values triggered in 66cl4‐ NPNT cells in comparison with 66cl4‐ EV cells. The blue circle, ‘ EV rm NPNT vs EV ’, represents 66cl4‐ EV cells cultured on rm NPNT ( EV rm NPNT ) in comparison with 66cl4‐ EV cells seeded in noncoated wells. The purple circle represents proteins regulated by the integrin‐binding motifs of NPNT ; the effect of a single mutation in the RGD motif ( RGD → RGE ) versus mutations in both RGD and EIE motifs ( RGD ‐ EIE ‐> RGE ‐ AIA ). (B) Box plot showing log2 protein abundance of the four overlapping proteins from the Venn diagram.

    Journal: FEBS Open Bio

    Article Title: Nephronectin mediates p38 MAPK ‐induced cell viability via its integrin‐binding enhancer motif

    doi: 10.1002/2211-5463.12544

    Figure Lengend Snippet: Reverse‐phase protein array analysis of NPNT ‐mediated signaling. The Venn diagram includes number of proteins significantly regulated and/or modified ( P < 0. 05) in all four biological replicates. (A) The pink circle in the Venn diagram, ‘ NPNT vs EV ’, denotes the log‐fold change values triggered in 66cl4‐ NPNT cells in comparison with 66cl4‐ EV cells. The blue circle, ‘ EV rm NPNT vs EV ’, represents 66cl4‐ EV cells cultured on rm NPNT ( EV rm NPNT ) in comparison with 66cl4‐ EV cells seeded in noncoated wells. The purple circle represents proteins regulated by the integrin‐binding motifs of NPNT ; the effect of a single mutation in the RGD motif ( RGD → RGE ) versus mutations in both RGD and EIE motifs ( RGD ‐ EIE ‐> RGE ‐ AIA ). (B) Box plot showing log2 protein abundance of the four overlapping proteins from the Venn diagram.

    Article Snippet: The effect of incubating 66cl4‐EV cells with 2 μg·mL −1 recombinant mouse NPNT (rmNPNT) (R&D systems, Minneapolis, MN, USA; Cat: 4298‐NP‐050) in PBS for 1 h prior fixing was also investigated.

    Techniques: Protein Array, Modification, Comparison, Cell Culture, Binding Assay, Mutagenesis, Quantitative Proteomics

    Top predicted molecular and cellular functions. RPPA results from RGE vs RGE‐AIA group were analyzed using the web‐based software application ingenuity pathway analysis (IPA) tool to identify the most significant NPNT‐responsive functions

    Journal: FEBS Open Bio

    Article Title: Nephronectin mediates p38 MAPK ‐induced cell viability via its integrin‐binding enhancer motif

    doi: 10.1002/2211-5463.12544

    Figure Lengend Snippet: Top predicted molecular and cellular functions. RPPA results from RGE vs RGE‐AIA group were analyzed using the web‐based software application ingenuity pathway analysis (IPA) tool to identify the most significant NPNT‐responsive functions

    Article Snippet: The effect of incubating 66cl4‐EV cells with 2 μg·mL −1 recombinant mouse NPNT (rmNPNT) (R&D systems, Minneapolis, MN, USA; Cat: 4298‐NP‐050) in PBS for 1 h prior fixing was also investigated.

    Techniques: Software, Activation Assay

    Nephronectin mediates cell viability via p38 signaling pathways. (A) Indicated variants of 66cl4 cells were treated with (±) 4 μ m p38 MAPK inhibitor ( BIRB 796) for 24 h, in addition to serum deprivation. Where indicated, 66cl4‐ EV cells were stimulated by adding 2 μg·mL −1 rm NPNT to the cell culture medium. Cell viability was determined using CellTiter‐Glo. (B) Viability of NPNT expressing, 4T1 cells with a NPNT ‐targeted short hairpin (sh‐ NPNT ) and a nontargeting sh RNA (sh‐ctr) was tested using CellTiter‐Glo. Significance is tested using a two‐tailed Student's t‐test. * P < 0. 05, ** P < 0. 005, *** P < 0. 0001. Error bars represent SD . N = number of independent experiments, n = total number of replicates in each test group. (C) Illustration summarizing the cellular effects of integrin binding to wild‐type or mutated NPNT via p38 MAPK .

    Journal: FEBS Open Bio

    Article Title: Nephronectin mediates p38 MAPK ‐induced cell viability via its integrin‐binding enhancer motif

    doi: 10.1002/2211-5463.12544

    Figure Lengend Snippet: Nephronectin mediates cell viability via p38 signaling pathways. (A) Indicated variants of 66cl4 cells were treated with (±) 4 μ m p38 MAPK inhibitor ( BIRB 796) for 24 h, in addition to serum deprivation. Where indicated, 66cl4‐ EV cells were stimulated by adding 2 μg·mL −1 rm NPNT to the cell culture medium. Cell viability was determined using CellTiter‐Glo. (B) Viability of NPNT expressing, 4T1 cells with a NPNT ‐targeted short hairpin (sh‐ NPNT ) and a nontargeting sh RNA (sh‐ctr) was tested using CellTiter‐Glo. Significance is tested using a two‐tailed Student's t‐test. * P < 0. 05, ** P < 0. 005, *** P < 0. 0001. Error bars represent SD . N = number of independent experiments, n = total number of replicates in each test group. (C) Illustration summarizing the cellular effects of integrin binding to wild‐type or mutated NPNT via p38 MAPK .

    Article Snippet: The effect of incubating 66cl4‐EV cells with 2 μg·mL −1 recombinant mouse NPNT (rmNPNT) (R&D systems, Minneapolis, MN, USA; Cat: 4298‐NP‐050) in PBS for 1 h prior fixing was also investigated.

    Techniques: Protein-Protein interactions, Cell Culture, Expressing, Two Tailed Test, Binding Assay