- ¥1740
- Sigma-Aldrich
- 进口
- 14533-100MG
- 2025年09月10日
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- 详细信息
- 文献和实验
- 技术资料
- 保存条件:
2-8°C
- 保质期:
根据瓶身LOT号查询
- 英文名:
bisBenzimide H 33342 trihydrochloride
- 库存:
有现货
- 供应商:
浙江羽翔生物科技有限公司
- CAS号:
23491-52-3
- 规格:
100MG
属性
质量水平
200
方案
≥97.0% (HPLC)
荧光
λex 340 nm; λem 510 nm
λex 355 nm; λem 465 nm in TE buffer; DNA
适用性
suitable for fluorescence
储存温度
2-8°C
SMILES字符串
Cl[H].Cl[H].Cl[H].CCOc1ccc(cc1)C2=NCc3cc(ccc3N2)C4=NCc5cc(ccc5N4)N6CCN(C)CC6
InChI
1S/C29H32N6O.3ClH/c1-3-36-25-8-4-20(5-9-25)28-30-18-22-16-21(6-10-26(22)32-28)29-31-19-23-17-24(7-11-27(23)33-29)35-14-12-34(2)13-15-35;;;/h4-11,16-17H,3,12-15,18-19H2,1-2H3,(H,30,32)(H,31,33);3*1H
InChI key
FYEVKHPLBHLWHK-UHFFFAOYSA-N
应用
最大激发波=346nm
最大发射波长=460nm
生化/生理作用
包装
其他说明
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文献和实验Targeting a therapeutic LIF transgene to muscle via the immune system ameliorates muscular dystrophy.
Many potentially therapeutic molecules have been identified for treating Duchenne muscular dystrophy. However, targeting those molecules only to sites of active pathology is an obstacle to their clinical use. Because dystrophic muscles become extensively inflamed, we tested whether expressing a therapeutic transgene in leukocyte progenitors that invade muscle would provide selective, timely delivery to diseased muscle. We designed a transgene in which leukemia inhibitory factor (LIF) is under control of a leukocyte-specific promoter and transplanted transgenic cells into dystrophic mice. Transplantation diminishes pathology, reduces Th2 cytokines in muscle and biases macrophages away from a CD163+/CD206+ phenotype that promotes fibrosis. Transgenic cells also abrogate TGFβ signaling, reduce fibro/adipogenic progenitor cells and reduce fibrogenesis of muscle cells. These findings indicate that leukocytes expressing a LIF transgene reduce fibrosis by suppressing type 2 immunity and highlight a novel application by which immune cells can be genetically modified as potential therapeutics to treat muscle disease.
通用,尤其是在进行动态检查时。医琳师妹:我将我所作的方法与大家共享:吖啶橙/溴化乙锭双荧光染色测定PC12细胞凋亡(acridine orange/ethidium bromide, AO/EB):(1)细胞爬片:在6孔培养板中预先置入玻璃盖玻片,接种细胞悬液,干预后,予95%乙醇固定15分钟,微干,然后准备荧光染色。将100mg/L溶于PBS的吖啶橙和100mg/L溶于PBS的溴化乙锭各5μl(临用前混合加入,加样量宜小,有时各2μl-5μl足够,量太大容易形成细胞凋亡的假阳性),在照相前混匀
双苯咪唑类的Hochest-33342和33258及 JC-1染色
可直接离心收集(1 000r/min,5min)。对于贴壁生长的细胞可以先收集细胞培养液(可能含有因凋亡而悬浮的细胞),再用胰酶消化贴壁细胞,然后将两者合并,离心收集细胞并用1×PBS洗细胞沉淀物。 (3)固定:细胞沉淀物悬浮在300ul甲醛(4%)中固定30min,然后经PBS洗涤后离心收获细胞。 (4)染色:细胞在100ul Hoechst-33342(sigma)中染色10min,然后将细胞悬液滴在载片上,盖上盖玻片,用荧光显微镜观察并拍照
【摘要】目的 构建和表达抗CD3/抗Pgp微型双功能抗体,并测定该微型双功能抗体的生物学活性。方法 采用PCR和overlap PCR方法构建抗CD3/抗CD20微型双功能抗体,并用双脱氧终止法测定DNA序列;采用亲和层析法纯化该产物,并用Western blot和分子排阻层析鉴定纯化产物;采用免疫荧光法、放射免疫分析法和玫瑰花环试验鉴定纯化产物与靶细胞的结合活性。结果 DNA序列测定结果表明:抗CD3/抗Pgp微型双功能抗体已构建成功,表达可溶性产物的产量达2mg/l以上,纯化产物中二
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