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Boston Biochem/Human Phospho-Ubiquitin (S65) Antibody/A-110

价格
¥5980.00
货号:A-110
浏览量:127
品牌:Boston Biochem
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SummaryData ExamplesPreparation and StorageReconstitution CalculatorBackgroundProduct DatasheetsRelated Research Areas

Human Phospho-Ubiquitin (S65) Antibody Summary

Specificity
This antibody detects mono- and poly-Ubiquitin chains that are phosphorylated on Serine 65. It has no cross-reactivity with non-phosphorylated Ubiquitin, Ubiquitin phosphorylated at Serine 57 or Tyrosine 59, or phosphorylated Parkin. Detects only recombinant, phosporylated Ubiquitin. Not recommended on natural lysates (see western blot results below).
Source
Polyclonal Rabbit IgG
Purification
Antigen Affinity-purified
Immunogen
Peptide sequence from Ubiquitin, phosphorylated at Serine 65. Accession # P0CG47
Formulation
0.5 mg/ml in PBS pH 7.4, 50% (v/v) Glycerol
Label
Unconjugated

Applications

Recommended Concentration
Sample
Western Blot
0.5-1 µg/mL
See below

Please Note: Optimal dilutions should be determined by each laboratory for each application.General Protocolsare available in the Technical Information section on our website.

Data Examples

Western BlotDetection of Phospho-Ubiquitin (S65) by Western blot.View Larger

Detection of Phospho-Ubiquitin (S65) by Western blot.Tetraubiquitin chains of each indicated linkage type were incubated for 0-4 hours in reactions containing recombinant PINK1 kinase (Cat# AP-180) and ATP. At indicated times a portion of each reaction was removed and terminated with SDS-PAGE sample buffer. SDS-PAGE gels (10-20%) were used to resolve approximately 150 ng of Ubiquitin tetramer from each reaction. Western Blots were developed using eitheralpha -phospho-Ubiquitin, pS65 (upper panels) or anti-Ubiquitin (Cat# MAB701, lower panel). Primary antibodies were used at 1 μg/ml in PBST + 0.5% BSA, while HRP-labeled secondary antibodies ( alpha -rabbit for A-110,alpha -mouse for MAB701) were used at a 1:10,000 dilution in PBST + 0.5% BSA. Further details are available upon request.

Western BlotDetection of Phospho-Ubiquitin (S65) by Western blot.View Larger

Detection of Phospho-Ubiquitin (S65) by Western blot.Tetraubiquitin chains of each indicated linkage type were incubated for 0-4 hours in reactions containing recombinant PINK1 kinase (Cat# AP-180) and ATP. At indicated times a portion of each reaction was removed and terminated with SDS-PAGE sample buffer. SDS-PAGE gels (10-20%) were used to resolve approximately 150 ng of Ubiquitin tetramer from each reaction. Western Blots were developed using eitheralpha -phospho-Ubiquitin, pS65 (upper panels) or anti-Ubiquitin (Cat# MAB701, lower panel). Primary antibodies were used at 1 μg/ml in PBST + 0.5% BSA, while HRP-labeled secondary antibodies ( alpha -rabbit for A-110,alpha -mouse for MAB701) were used at a 1:10,000 dilution in PBST + 0.5% BSA. Further details are available upon request.

Reconstitution Calculator

Reconstitution Calculator

The reconstitution calculator allows you to quickly calculate the volume of a reagent to reconstitute your vial. Simply enter the mass of reagent and the target concentration and the calculator will determine the rest.

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Preparation and Storage

Shipping
The product is shipped with polar packs. Upon receipt, store it immediately at the temperature recommended below.
Stability & Storage
  • 6 months from date of receipt, -20 °C as supplied.
  • 3 months, -20 °C under sterile conditions after opening.

Background: Ubiquitin

Serine/Threonine kinase PINK1 (PTEN-induced putative kinase protein 1) plays a critical role in preventing mitochondrial dysfunction during cellular stress. PINK is translated in the cytosol, then translocated to the outer mitochondrial membrane where it is rapidly cleaved and degraded as a part of normal mitochondrial function. In damaged (depolarized) mitochondria PINK becomes stabilized and accumulates, resulting in the subsequent phosphorylation of numerous proteins on the mitochondrial surface including Mfn2. Ultimately PARK2 (E3 Ubiquitin Ligase Parkin) is recruited to the damaged mitochondria where it is activated by PINK-mediated phosphorylation of PARK2 at serine 65, and PARK2 interaction with phosphorylated Ubiquitin (also phosphorylated by PINK on serine 65). This signaling cascade is critical for clearing the damaged mitochondria via selective autophagy (mitophagy) by mediating activation and translocation of PARK2.

Entrez Gene IDs
7314 (Human); 298693 (Rat)
Alternate Names
RPS27A; UBA52; UBB ubiquitin B; UBB; UBC; Ubiquitin

Product Datasheets

Product Datasheet
COA

FAQs

No product specific FAQs exist for this product, however you may

View all Antibody FAQs

Isotype Controls

Normal Rabbit IgG Control

AB-105-C
51Citations
10Reviews
1Image
Ctrl

Normal RabbitIgG Control

MAB1050
1Image
Ctrl,CyTOF-ready

Secondary Antibodies

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1Citations
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Donkey Anti-Rabbit IgG NorthernLights™ NL493-conjugated Antibody

NL006
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Rabbit IgG PE-conjugated Antibody

F0110
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Rabbit IgG APC-conjugated Antibody

F0111
3Citations
2Reviews
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Donkey Anti-Rabbit IgG NorthernLights™ NL557-conjugated Antibody

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1Review
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Mouse/Rabbit IgG VisUCyte HRP Polymer Antibody

VC002
1Citations
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Rabbit IgG Fluorescein-conjugated Antibody

F0112
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Donkey Anti-Rabbit IgG (H+L) Antibody

D-301-C-ABS2

Rabbit IgG Biotinylated Antibody

BAF008
6Citations
3Reviews
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WB,Simple Western

Rabbit IgG HRP-conjugated Antibody

HAF008
52Citations
3Reviews
1Image
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Rabbit IgG VisUCyte HRP Polymer Antibody

VC003
1Image
IHC

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Boston Biochem波士顿生物化学已与IQ Proteomics™合作,为分析您的泛素化蛋白提供定制服务。使用哈佛医学院Gygi实验室开发的泛素绝对定量(AQUA)技术,我们可以对样品中存在的不同泛素连接进行定量表征。