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48-602MAG
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06-1002
Sigma-AldrichAnti-LAP2 Antibody
Anti-LAP2 Antibody is an antibody against LAP2 for use in WB, IC & IF.
More>>Anti-LAP2 Antibody is an antibody against LAP2 for use in WB, IC & IF. Less<<
Anti-LAP2 Antibody: SDB (Sicherheitsdatenblätter), Analysenzertifikate und Qualitätszertifikate, Dossiers, Broschüren und andere verfügbare Dokumente.
The inner membrane of the nuclear envelope is connected to the nuclear lamina. The main components of the nuclear lamina are Type V intermediate filaments called lamins and lamin binding proteins including lamin B receptor, emerin, MANI, LAP1 (3 isoforms), and LAP2 (several isoforms). The lamins are divided into two groups: the constitutively expressed lamin B and the developmentaly regulated lamin A. The best characterized isoforms of lamin binding protein LAP2 are LAP2α and LAP2β. LAP2β is a type II membrane protein in the inner nuclear membrane that binds lamin B and is important to cell viability and controlling nuclear lamina growth. LAP2α has been characterized as a nucleoplasmic protein that interacts with A-type lamins to control gene expression, transcription, and chromatin organization.
References
Product Information
Format
Affinity Purified
Control
HeLa cell lysate
Presentation
Purified rabbit polyclonal in buffer containing 0.1 M Tris-Glycine, (pH 7.4), 150 mM NaCl, with 0.05% sodium azide.
Anti-LAP2 Antibody is an antibody against LAP2 for use in WB, IC & IF.
Key Applications
Western Blotting
Immunocytochemistry
Immunofluorescence
Application Notes
Immunofluorescence: Representative lot data. This antibody was used to detect the nuclear lamina by immunofluorescence.
Immunocytochemistry: Representative lot data. A previous lot was used in confocal fluorescent analysis of A431, HeLa and NIH/3T3 cells using anti-LAP2 rabbit polyclonal antibody (Red). Actin filaments have been labeled with AlexaFluor® 488 -Phalloidin (Green). Nuclear is stained with DAPI (Blue). Positive nuclear staining.
Biological Information
Immunogen
KLH-conjugated synthetic linear peptide corresponding to LAP2.
Host
Rabbit
Specificity
This antibody recognizes LAP2.
Species Reactivity
Human
Canine
Mouse
Rat
Species Reactivity Note
Tested on human and mouse. Predicted to cross-react with canine (dog) and rat based on sequence homology.
FUNCTION: May help direct the assembly of the nuclear lamina and thereby help maintain the structural organization of the nuclear envelope. Possible receptor for attachment of lamin filaments to the inner nuclear membrane. May be involved in the control of initiation of DNA replication through its interaction with NAKAP95.
TP and TP5 may play a role in T-cell development and function. TP5 is an immunomodulating pentapeptide.
SUBUNIT STRUCTURE: Interacts with LMNB1, LMNB2, BANF1, NAKAP95, GMCL and chromosomes By similarity.
SUBCELLULAR lOCATION: Nucleus inner membrane; Single-pass type II membrane protein. Note= Tightly associated with the nuclear lamina.
TISSUE SPECIFICTY: Expressed in many tissues. Most abundant in adult thymus and fetal liver.
DOMAIN: Has two structurally independent, non-interacting domains: LEM-like (also called LAP2-N or LEM-D) and LEM (also called LAP2-C or LEM-B). LEM-like binds DNA while LEM interacts with BANF1.
PTM: Mitosis-specific phosphorylation specifically abolishes its binding to lamin B and chromosomes By similarity.
PHARMACEUTICAL USE: TP5 is available under the names Timunox (Cilag), Sintomodulina (Italofarmaco) and Mepentil (Recordati). Used in primary and secondary immune deficiencies, autoimmunity, infections and cancer.
SIMILARITY: Belongs to the LEM family.
Contains 1 LEM domain.
Contains 1 LEM-like domain.
Molecular Weight
~55 kDa
Physicochemical Information
Dimensions
Materials Information
Toxicological Information
Safety Information according to GHS
Safety Information
Product Usage Statements
Quality Assurance
Evaluated by western blot on HeLa cell lysate.
Western Blot Analysis: A 1:1000-1:3000 dilution of this antibody was used to detect LAP2 in HeLa cell lysate.
Usage Statement
Unless otherwise stated in our catalog or other company documentation accompanying the product(s), our products are intended for research use only and are not to be used for any other purpose, which includes but is not limited to, unauthorized commercial uses, in vitro diagnostic uses, ex vivo or in vivo therapeutic uses or any type of consumption or application to humans or animals.
Disruption of cell cycle regulation is one mechanism proposed for how nuclear envelope protein mutation can cause disease. Thus far only a few nuclear envelope proteins have been tested/found to affect cell cycle progression: to identify others, 39 novel nuclear envelope transmembrane proteins were screened for their ability to alter flow cytometry cell cycle/DNA content profiles when exogenously expressed. Eight had notable effects with seven increasing and one decreasing the 4N:2N ratio. We subsequently focused on NET4/Tmem53 that lost its effects in p53(-/-) cells and retinoblastoma protein-deficient cells. NET4/TMEM53 knockdown by siRNA altered flow cytometry cell cycle/DNA content profiles in a similar way as overexpression. NET4/TMEM53 knockdown did not affect total retinoblastoma protein levels, unlike nuclear envelope-associated proteins Lamin A and LAP2α. However, a decrease in phosphorylated retinoblastoma protein was observed along with a doubling of p53 levels and a 7-fold increase in p21. Consequently cells withdrew from the cell cycle, which was confirmed in MRC5 cells by a drop in the percentage of cells expressing Ki-67 antigen and an increase in the number of cells stained for ß-galactosidase. The ß-galactosidase upregulation suggests that cells become prematurely senescent. Finally, the changes in retinoblastoma protein, p53, and p21 resulting from loss of NET4/Tmem53 were dependent upon active p38 MAP kinase. The finding that roughly a fifth of nuclear envelope transmembrane proteins screened yielded alterations in flow cytometry cell cycle/DNA content profiles suggests a much greater influence of the nuclear envelope on the cell cycle than is widely held.
