|
Malondialdehye
(MDA), 4-Hydroxy-2-Nonenal (HNE), Nitrated Tyrosine
and 8-hydroxyguanosine (8-OHG), and S-Nitroso-Cys (SNO-Cys) Antibodies
|
Items |
Antigen |
Ab
Host |
Species reactivity |
Antiserum
Cat # 100 ul |
Aff Pure IgG/Mono
Cat # 100 ug |
|
MDA Compound
For modifiction of proteins |
Malondialdehyde (MDA)-bis(dimethyl acetal)
solution
Cat # MDA51-10; 10 ml |
|
Anti-MDA (ab # 1) |
MDA-KLH |
Poly, Rb |
All species |
MDA11-S |
|
|
Anti-MDA (ab # 2) |
MDA-KLH |
Poly, G |
All species |
MDA12-S |
|
|
HNE Related Products
|
|
HNE-Compound
For modification of proteins |
4 hydroxynonenal (HNE), >98% pure;
Cat # HNE51-5; 5 mg
4 hydroxynonenal (HNE), >98% pure; Cat #
HNE51-10; 10 mg |
|
Anti-HNE (ab # 1) |
HNE-KLH |
Poly, Rb |
All species |
HNE11-S |
|
|
HNE-BSA Conjugate control #1
|
For Western blot (supplied in Sample buffer,
reduced), Cat # HNE11-C; 100 ul |
|
Anti-HNE (ab # 2)
|
HNE-KLH |
Poly, G
|
all species |
HNE12-S |
|
|
HNE-BSA Conjugate control #2
|
For Western blot (supplied in
Sample buffer, reduced), Cat # HNE12-C; 100 ul
|
|
HNE-BSA Conjugate control #2
|
For ELISA, stds or WB (supplied in
PBS buffer), Cat # HNE15-R; 100 ug
|
|
Nitrotyrosine Related Products
|
|
Nitrated-Tyrosine
(ab # 1) |
Nitrated-KLH |
mouse
mono |
all species |
|
NITT11-M |
|
Nitrated-Tyrosine
(ab # 2) |
Nitrated-KLH |
Poly, Rb |
all species |
|
NITT12-A |
|
Nitrated-Tyrosine
(ab # 3) |
Nitrated-KLH |
Poly, G |
all species |
NITT13-S |
|
|
Nitrated Proteins control |
Nitrated Mol. Wt protein Standard for
Western, Cat # NITT12-C, 100 ul |
|
Nitrated Proteins control
|
Nitrated BSA
protein For Standard or ELISA etc, Cat # NITT15-N,
100 ug
Nitrated Ovalbumin protein For
Standard or ELISA etc, Cat # NITT16-N, 100 ug
|
|
Nitroso-Cysteine
(SNO-Cys) |
Nitroso-Cysteine
-KLH |
Poly, Rb |
all species |
. |
NISC11-A |
|
S-Nitrosoylated-BSA protein
Conjugate (Control) |
S-Nitrosoylated-BSA Protein
Conjugate for ELISA or antibody blocking
Cat # SNOBSA-N-100 (100 ug)
|
|
8-OH Guanosine Related Products
|
|
8-Hydroxyguanosine Chemical |
8OHG |
8-Hydroxy Guanosine ;
Cat # 8OHG15-N-1; 1 mg
8-Hydroxy Guanosine ; Cat # 8OHG15-N-5; 5
mg |
|
8-Hydroxyguanosine (8-OHG) ab # 1 |
8OHG-BSA/ |
M, mono |
all species |
|
8OHG11-M |
|
8-Hydroxyguanosine (8-OHG) ab # 2 |
8OHG-BSA |
Poly, G |
all species |
8OHG12-S |
|
M= Mouse; R=Rat; H=Human; Rb=Rabbit; G=goat; B=Bovine, MO=Monkey; P=pig; CT=
near C-terminus; NT=near N-terminus; Internal=Middle of protein.
EC=extracellular; CP=cytoplasmic domains *
Malondialdehye (MDA), 4-Hydroxy-2-Nonenal (HNE), Nitrated Tyrosine and
8-hydroxyguanosine (8-OHG), and S-Nitroso-Cys (SNO-Cys) Antibodies-General
Information
MDA is a physiological compound produced
by peroxidative decomposition of unsaturated lipids as a by-product of
arachidonic metabolism. Under normal conditions, MDA is quickly oxidized to
acetate or malonate and then to CO2 via TCA cycle. Excessive production of
MDA, as a result of tissue injury and DNA-damage, could combine with free
amino groups of proteins resulting into MDA-modified protein adducts.
Modifications of proteins by MDA could conceivably alter biological
properties of proteins. Moreover, MDA-modified protein may serve as an
antigen and invoke production of autoantibodies and subsequent destruction
of MDA-modified proteins. An uncontrolled diabetes mellitus is known to be
associated with high free radical activity. Injections if streptozotocin has
been shown to induce MDA-modified proteins in the plasma. MDA-modified LDL
shows altered behavior and is entrapped in arterial walls. Autoantibodies to
MDA-LDL have been detected in human and rabbits sera. Moreover, alcohol fed
rats and alcoholics have autoantibodies to acetaldehyde. Further progress in
this field is hampered by the availability of anti-MDA antibodies.
Among the aldehyde which originate from the peroxidation of cellular
membrane lipids, 4-hydroxy-2-nonenal (HNE) is
the major aldehyde generated by free radical attack on w-6 polyunsaturated
fatty acids. HNE is largely responsible for pathogenesis during oxidative
stress. HNE is highly reactive towards free sulfydryl groups of proteins
producing thioether adducts that further undergo cyclization to form
hemiacetals. HNE also reacts with histidine and lysine residues of proteins
to form stable Michael addition-type adducts. HNE induces heat shock
protein, inhibits cellular proliferation and highly toxic to cells. It
exhibits genotoxic and mutagenic effects as well. Elevated levels of HNE
modified nigral neurons were also observed in Parkinson disease.
Reactive oxygen species (ROS) are formed at high levels as by-products of
the normal cellular metabolism. Both nuclear and Mitochondrial DNA has been
shown to accumulate high levels of 8-hydroxy-2'-deoxyguanosine, a very
stable and damaging product of hydroxylation of guanine at carbon 8.
8-hydroxyguanosine (8-OHG) induces transversion
of G to T, which is potentially mutagenic. The base excision repair (BER)
pathway is the most important cellular protection mechanism responding to
oxidative DNA damage. They remove modified DNA bases before they are
incorporated into DNA during replication. The key enzymes MutT homologs
(MutT/MTH) in the BER process are DNA glycosylases, which remove different
damaged bases by cleavage of the N-glycosylic bonds between the bases and
the deoxyribose moieties of the nucleotide residues. The 8-oxoG glycosylases
(Fpg or MutM/OGG) and the MutY homologs (MutY/MYH) glycosylases along with
MutT/MTH protect cells from the mutagenic effects of 8-oxoG.
8-hydroxyguanosine (8-OHG) has been used as oxidative stress marker.
Nitric oxide (NO) and reactive oxygen species (ROS) are important mediators
to produce harmful or protective functions. NO can react with superoxide
anions (O2.-), yielding the toxic oxidizing agent peroxynitrite (ONOO-).
Peroxynitrite induces nitration of tyrosine residues
leading to changes of protein structure
and function, and alterations in signaling pathways. Antibodies to
nitrotyrosine have been used to monitor the status of peroxynitrite-induced
modification of proteins.
S-nitrosylation of cysteine thiols in proteins
by the highly labile NO radical has been identified as a important effectors
of NO-related bioactivity both in NOS-containing cells and intercellular
signaling. Most cells contain low levels of nitrosylated proteins that are
thought to be regulated by S-nitrosylation and denitrosylation.
S-nitrosylation of proteins serves as a ubiquitous post-translational
modification that dynamically regulates a broad functional spectrum of
proteins. The majority of these proteins are regulated by S-nitrosylation on
a single critical cysteine residue within an acidic/basic or hydrophobic
structural motif that may also be subject to oxygen- or
glutathione-dependent modification. NO-sensitive ion channels including the
cardiac and skeletal muscle ryanodine receptor (RyR1), N-methyl-D-aspartate
receptor (NMDAR) complex, cyclic-nucleotide gated ion channel, are modulated
by S-nitrosylation. S-nitrosylation of capsase-3 inhibits apoptosis
signaling. S-nitrosylation activates matrix metalloproteinase-9 (MMP-9) and
induces neuronal apoptosis. The small G-protein p21Ras and Jun kinase are
regulated by S-nitrosylation. The activity of transcription factors such as
NF?B, c-jun, and c-fos is modulated by S-nitrosylation. In addition, the
formation of S-nitrosylated glutathione (GSNO) has been proposed to be one
of the major storage forms of NO in vivo.
All Products are for in vitro research use only.
rev 50105A |