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Megazyme/1,2-α-L-Fucosidase (microbial)?/E-FUCM/3 Units at 37

Megazyme/1,2-α-L-Fucosidase (microbial)?/E-FUCM/3 Units at 37


商品編號


E-FUCM



品牌


Megazyme



公司


Megazyme



公司分類(lèi)


Enzymes



Size

3 Units at 37
o
C

商品信息

High purity recombinant?1,2-α-L-Fucosidase (microbial) for use in research, biochemical enzyme assays and
in vitro
diagnostic analysis.?

EC 3.2.1.63
CAZy Family: GH95
CAS:
37288-45-2

1,2-alpha-L-fucosidase; 2-alpha-L-fucopyranosyl-beta-D-galactoside fucohydrolase

Recombinant.
From a

microbial source
.
In solution (Tris.HCl/NaCl/EDTA).
Supplied at ~ 12 U/mL.?

Specific activity:

~ 160 U/mg (37
o
C, pH 6.5 on 2’-fucosyllactose)

St
ABI
lity:
? >?3 years at 4
o
C.



Comparisons of
Caenorha
BD
itis
fucosyltransferase mutants reveal a multiplicity of isomeric N-glycan structures.

Yan, S., Jin, C., Wilson, I. B. & Paschinger, K. (2015).
Journal of Proteome Research
, 14(12), 5291-5305.


Link to Article

Read Abstract

Recent studies have shown a remarkable degree of plasticity in the N-glycome of the model nematode
Caenorha
BD
itis elegans
; ablation of glycosylation-relevant genes can result in r
ADI
cally altered N-glycan profiles despite only minor
BIOLOG
ical phenotypic effects. Up to four fucose residues and five different linkages of fucose are known on the N-glycans of
C. elegans
. Due to the complexity in the wild type, we established three mutant strains defective in two core fucosyltransferases each (
fut-1;fut-6
,
fut-1;fut-8
, and
fut-6;fut-8
). Enzymatically released N-glycans were subject to HPLC and MALDI-TOF MS/MS, in combination with various treatments, to verify structural details. The N-glycome of the
fut-1;fut-6
mutant was the most complex of the three double-mutant strains due to the extension of the core α1,6-fucose as well as the presence of fucose on the bisecting galactose. In contrast, maximally two fucoses were found on N-glycans of the
fut-1;fut-8
and
fut-6;fut-8
strains. The different locations and capping of fucose meant that up to 13 isomeric structures, many highly galactosylated, were determined for some single masses. These data not only show the high vari
ABI
lity of the N-glycomic capacity of a “simple” nematode but also exemplify the need for multiple approaches to reveal individual glycan structures within complex invertebrate glycomes.





Analysis of Invertebrate and Protist
N
-Glycans.

Hykollari, A., Paschinger, K., Eckmair, B. & Wilson, I. B. (2017).
High-Throughput Glycomics and Glycoproteomics: Methods and Protocols
, 1503, 167-184.


Link to Article

Read Abstract

N-glycans from invertebrates and protists have often unusual structures which present analytical challenges. Both core and antennal modifications can be quite different from the more familiar vertebrate glycan motifs; thereby, contrary to the concept that “simple” organisms have “simple” N-glycans, rather complex oligosaccharides structures, including zwitterionic and anionic ones, have been found in a range of species. Thus, to facilitate the optimized elucidation of the maximal poss
IBL
e range of structures, the analytical workflow for glycomics of these organisms should include sequential release and fractionation steps. Peptide:N-glycosidase F is sufficient to isolate N-glycans from fungi and some protists, but in most invertebrates core α1,3-fucose is present, so release of the glycans from glycopeptides with peptide:N-glycosidases A is required. Subsequent solid-phase extraction with graphitized carbon and reversed phase resins enables different classes of N-glycans to be separated prior to high-pressure liquid chromatography (HPLC) and matrix-assisted laser desorption/ionization time-of-flight mass spectrometry (MALDI-TOF MS). Depending on the types and numbers of glycans present, either reversed- or normal-phase HPLC (or both in series) enable even single isomeric or isobaric structures to be separated prior to MALDI-TOF MS and MS/MS. The use of enzymatic or chemical treatments allows further insights to be gained, although some glycan modifications (especially methylation) are resistant. Using a battery of methods, sometimes up to 100 structures from a single organism can be assigned, a complexity which raises evolutionary questions regarding the function of these glycans.









DESCRIPTION

1,2-α-L-Fucosidase (microbial)

EC 3.2.1.63
CAZy Family: GH95
CAS:?
37288-45-2

Synonyms:
1,2-alpha-L-fucosidase; 2-alpha-L-fucopyranosyl-beta-D-galactoside fucohydrolase

Form:
In solution (Tris.HCl/NaCl/EDTA).

St
ABI
lity
:
?
> 3 years at 4
o
C.

Specific activity
:
~ 160 U/mg (37
o
C, pH 6.5 on 2’-fucosyllactose).

Unit definition:
One Unit

of α-1,2-L-fucosidase activity is defined as the amount of enzyme required to release one μmol of α-L-fucose per minute from 2’-fucosyllactose (2 mM) in sodium phosphate buffer (100 mM), pH 6.5 at 37
o
C.

Specificity:
Highly specific for non-reducing terminal L-fucose residues linked to D-galactose residues by a 1,2-α-linkage. Does not hydrolyse
p
-nitrophenyl-α-L-fucopyranoside.

Applications:
For use in glyco
BIOLOG
y research.





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產(chǎn)品貨號:3138.7

3138.7 ¥
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