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92921-26-1
  • Sulfo-SMPB sodium

  • names:

    Sulfo-SMPB sodium

  • CAS號(hào):

    92921-26-1

    MDL Number: MFCD01861952
  • MF(分子式): C18H15N2NaO9S MW(分子量): 458.37
  • EINECS: Reaxys Number:
  • Pubchem ID:10274690 Brand:BIOFOUNT
Sulfo-SMPB sodium
Sulfo-SMPB sodium (92921-26-1)是一種不可降解 (non-cleavable) 的異雙功能化學(xué)交聯(lián)劑,含有 N-羥基丁二酰亞胺 (NHS) 酯和馬來酰亞胺基團(tuán),允許含胺和巰基的分子共價(jià)結(jié)合。
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中文別名 Sulfo-SMPB sodium(cas:92921-26-1)
英文別名 Sulfo-SMPB sodium(cas:92921-26-1),SULFO-SMPB,1-({4-[4-(2,5-Dioxo-2,5-dihydro-1H-pyrrol-1-yl)phenyl]butanoyl}oxy)-2,5-dioxo-3-pyrrolidinesulfonic acid
CAS號(hào) 92921-26-1
Inchi InChI=1S/C18H16N2O9S/c21-14-8-9-15(22)19(14)12-6-4-11(5-7-12)2-1-3-17(24)29-20-16(23)10-13(18(20)25)30(26,27)28/h4-9,13H,1-3,10H2,(H,26,27,28)
InchiKey VHYRLCJMMJQUBY-UHFFFAOYSA-N
分子式 Formula C18H15N2NaO9S
分子量 Molecular Weight 458.37
溶解度Solubility
性狀 Solid
儲(chǔ)藏條件 Storage conditions 請(qǐng)根據(jù)產(chǎn)品建議的存儲(chǔ)條件進(jìn)行存儲(chǔ),Please store the product under the recommended condition sin the description.
Sulfo-SMPB sodium(CAS:92921-26-1)實(shí)驗(yàn)注意事項(xiàng):
1.實(shí)驗(yàn)前需戴好防護(hù)眼鏡,穿戴防護(hù)服和口罩,佩戴手套,避免與皮膚接觸。
2.實(shí)驗(yàn)過程中如遇到有毒或者刺激性物質(zhì)及有害物質(zhì)產(chǎn)生,必要時(shí)實(shí)驗(yàn)操作需要手套箱內(nèi)完成以免對(duì)實(shí)驗(yàn)人員造成傷害
3.實(shí)驗(yàn)后產(chǎn)生的廢棄物需分類存儲(chǔ),并交于專業(yè)生物廢氣物處理公司處理,以免造成環(huán)境污染Experimental considerations:
1. Wear protective glasses, protective clothing and masks, gloves, and avoid contact with the skin during the experiment.
2. The waste generated after the experiment needs to be stored separately, and handed over to a professional biological waste gas treatment company to avoid environmental pollution.
Tag:Sulfo-SMPB sodium 蒸汽壓,Sulfo-SMPB sodium 合成,Sulfo-SMPB sodium 標(biāo)準(zhǔn),Sulfo-SMPB sodium 應(yīng)用,Sulfo-SMPB sodium 合成,Sulfo-SMPB sodium 沸點(diǎn),Sulfo-SMPB sodium 閃點(diǎn),Sulfo-SMPB sodium 用途,Sulfo-SMPB sodium 溶解度,Sulfo-SMPB sodium 價(jià)格,Sulfo-SMPB sodium 作用
產(chǎn)品說明 Sulfo-SMPB sodium (92921-26-1)是一種不可降解 (non-cleavable) 的異雙功能化學(xué)交聯(lián)劑.
IntroductionSulfoMPB sodium(92921-26-1) is a nonleavable, heterobifunctional chemical crossinking reagent which contains Nydroxysuccinimide (NHS) ester and maleimide groups
Application1
Application2
Application3
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1.The murine haemopexin receptor. Evidence that the haemopexin-binding site resides on a 20 kDa subunit and that receptor recycling is regulated by protein kinase C/PMID 1646599; The Biochemical journal 1991 Jun; 276 ( Pt 2)(?):417-25/Name matches: smpb sulfosuccinimidyl 4-(p-maleimidophenyl)butyrate
Abstract:
Haemopexin receptors from mouse hepatoma (Hepa) cells were affinity-labelled by cross-linking to haem-125I-haemopexin complexes using two homo-[disuccinimidyl suberate (DSS) and 3,3'-dithiobis(succinimidyl propionate) (DTSSP)] and one hetero-[sulphosuccinimidyl 4-(p-maleimidophenyl)butyrate (sulpho-SMPB)] bifunctional cross-linking agents. Analysis of the cross-linked products by SDS/PAGE in the absence of reducing agents revealed that 125I-haemopexin was cross-linked specifically to a protein of apparent molecular mass 85-90 kDa. Upon reduction, haemopexin remained cross-linked to a protein of 20 kDa, suggesting that the murine haemopexin receptor has a subunit structure. Two subunits were identified: alpha (p65) and beta (p20). Furthermore, because haemopexin was cross-linked by all three agents to p20, the shortest cross-linker arm being 1.1 nm (11 A), we propose that the haem-haemopexin-binding site resides on this subunit. In addition, a cysteine residue of p20 is located near the haemopexin-binding site, since haemopexin, which has no free thiol groups, is cross-linked to this subunit by the hetero-bifunctional agent sulpho-SMPB. Exposure of Hepa cells to the tumour-promoting phorbol ester 4 alpha-phorbol 12-myristate 13-acetate (PMA) causes a rapid redistribution of haemopexin receptors from the cell surface to the cell interior. Within 2-4 min of incubation with 100 nM-PMA, there was an approx. 50% decrease in cell-surface haemopexin receptors, as judged by ligand binding at 0 degrees C and affinity labelling of the receptor. This time- and dose-dependent down-regulation was fully reversible within 60-90 min after removal of PMA, and the affinity of the remaining receptors was unaltered by PMA. The specificity of PMA was demonstrated by comparison with the non-tumour-promoter 4 alpha-phorbol, which did not affect any of the parameters examined. The amine H-7, a specific inhibitor of protein kinase C, antagonised the receptor redistribution effect of PMA, suggesting that the down-regulation of haemopexin receptors on the cell surface was a consequence of protein kinase C activation. The PMA-induced decrease in surface haemopexin receptors was due to a 2-fold increase in the rate of internalization (from 0.73 min-1 to 1.32 min-1), whereas the rate of exocytosis (0.6 min-1) was unchanged. PMA treatment, like binding of the natural ligand, haem-haemopexin, results in a lower steady-state level of surface haemopexin receptors independent of receptor synthesis, and the receptors were not degraded but were recycled back to the cell surface.
2.Covalent grafting of fibronectin onto plasma-treated PTFE: influence of the conjugation strategy on fibronectin biological activity/PMID 17457945; Macromolecular bioscience 2007 May; 7(5):738-45/Name matches: smpb sulfosuccinimidyl-4-(p-maleimidophenyl)butyrate
Abstract:Surface coating of synthetic materials is often considered to improve biomedical devices biocompatibility. In this study, we covalently bound fibronectin (FN) onto ammonia plasma-treated PTFE via two crosslinkers, namely glutaric anhydride (GA) and sulfosuccinimidyl-4-(p-maleimidophenyl)butyrate (sulfo-SMPB). With respect to clean PTFE, cell adhesion increased markedly on both FN grafted surfaces, although it was twice higher on PTFE-GA-FN than on PTFE-SMPB-FN. ELISA experiments performed with a polyclonal antibody revealed that the amount of FN is identical on both surfaces while monoclonal antibody specific to the RGD binding site clearly demonstrated a greater availability when FN is surface grafted through GA. These results provide evidence of a variation in protein conformation correlated with the surface conjugation strategy.
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