pspm 4.0 Search Results


np 40 lysis buffer  (Thermo Fisher)
99
Thermo Fisher np 40 lysis buffer
Np 40 Lysis Buffer, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 99 stars, based on 1 article reviews
np 40 lysis buffer - by Bioz Stars, 2026-06
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λ phosphatase  (New England Biolabs)
97
New England Biolabs λ phosphatase
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
λ Phosphatase, supplied by New England Biolabs, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 97 stars, based on 1 article reviews
λ phosphatase - by Bioz Stars, 2026-06
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nonidet p 40 lysis buffer  (Thermo Fisher)
99
Thermo Fisher nonidet p 40 lysis buffer
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Nonidet P 40 Lysis Buffer, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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np 40 buffer  (Bio-Rad)
98
Bio-Rad np 40 buffer
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Np 40 Buffer, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 98/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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np 40 lysis buffer  (Bio-Rad)
97
Bio-Rad np 40 lysis buffer
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Np 40 Lysis Buffer, supplied by Bio-Rad, used in various techniques. Bioz Stars score: 97/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/np 40 lysis buffer/product/Bio-Rad
Average 97 stars, based on 1 article reviews
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radioimmunoprecipitation ripa buffer  (Bio-Rad)
96
Bio-Rad radioimmunoprecipitation ripa buffer
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Radioimmunoprecipitation Ripa Buffer, supplied by Bio-Rad, 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/result/radioimmunoprecipitation ripa buffer/product/Bio-Rad
Average 96 stars, based on 1 article reviews
radioimmunoprecipitation ripa buffer - by Bioz Stars, 2026-06
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radioimmunoprecipitation assay buffer  (Thermo Fisher)
99
Thermo Fisher radioimmunoprecipitation assay buffer
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Radioimmunoprecipitation Assay Buffer, supplied by Thermo Fisher, 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/result/radioimmunoprecipitation assay buffer/product/Thermo Fisher
Average 99 stars, based on 1 article reviews
radioimmunoprecipitation assay buffer - by Bioz Stars, 2026-06
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streptavidin abc  (Agilent technologies)
99
Agilent technologies streptavidin abc
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Streptavidin Abc, supplied by Agilent technologies, 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/result/streptavidin abc/product/Agilent technologies
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streptavidin abc - by Bioz Stars, 2026-06
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alkaline phosphatase conjugated streptavidin  (Jackson Immuno)
94
Jackson Immuno alkaline phosphatase conjugated streptavidin
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Alkaline Phosphatase Conjugated Streptavidin, supplied by Jackson Immuno, used in various techniques. Bioz Stars score: 94/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/alkaline phosphatase conjugated streptavidin/product/Jackson Immuno
Average 94 stars, based on 1 article reviews
alkaline phosphatase conjugated streptavidin - by Bioz Stars, 2026-06
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ice cold chaps ip buffer  (Thermo Fisher)
99
Thermo Fisher ice cold chaps ip buffer
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Ice Cold Chaps Ip Buffer, supplied by Thermo Fisher, used in various techniques. Bioz Stars score: 99/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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Average 99 stars, based on 1 article reviews
ice cold chaps ip buffer - by Bioz Stars, 2026-06
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rabbit anti sp a polyclonal antibody  (Bioss)
92
Bioss rabbit anti sp a polyclonal antibody
Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with <t>λ</t> <t>phosphatase</t> (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.
Rabbit Anti Sp A Polyclonal Antibody, supplied by Bioss, used in various techniques. Bioz Stars score: 92/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/rabbit anti sp a polyclonal antibody/product/Bioss
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rabbit anti sp a polyclonal antibody - by Bioz Stars, 2026-06
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Image Search Results


Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with λ phosphatase (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.

Journal:

Article Title: Cell cycle regulation of Dfp1, an activator of the Hsk1 protein kinase

doi:

Figure Lengend Snippet: Expression and phosphorylation of Dfp1 during cell cycle progression. (A) A culture of the strain GBY398 was blocked in G2 and then released synchronously into the cell cycle. The culture was sampled every 15 min, and extracts were prepared. Dfp1 was detected by immunoblot analysis. The blot was reprobed for tubulin as a loading control. Synchrony was assessed by measuring the percentage of cells with a septum (% septation). The 60- (S) and 135-min (G2) samples are also shown side by side for comparison of the different Dfp1 isoforms. (B) Extracts were prepared from cells blocked in S phase (GBY397) or in G2 phase (GBY398) by using denaturing conditions. Proteins were immunoblotted, probing for Dfp1. (C) Native extracts were prepared from cells blocked in S or G2 phase. Hsk1 and associated Dfp1 were immunoprecipitated, and the immunoprecipitates were incubated with λ phosphatase (lanes 2), without λ phosphatase (lanes 3), or with λ phosphatase plus the inhibitor vanadate (lanes 4). The untreated controls are in lanes 1. Reaction products were subjected to immunoblot analysis, probing for Dfp1. Note that the fastest-migrating Dfp1 isoform seen in A and B is extracted inefficiently under native conditions. (D) The phosphorylation state of Dfp1 in S phase cells was analyzed in cds1+ or cds1Δ strains. Samples were taken from cultures arrested in S phase with hydroxyurea (+HU) or from asynchronous cultures (−HU). The position of the S phase Dfp1 phosphoisomer is indicated by the arrow.

Article Snippet: Immunoprecipitates were incubated with 40 units of λ phosphatase (New England Biolabs) for 15 min at 30°C.

Techniques: Expressing, Western Blot, Immunoprecipitation, Incubation