Cationic liposome-forming compound for transfection of DNA, RNA and other negatively charged molecules into eukaryotic cells. Mixing DOTAP with DNA results in spontaneously formed stable complexes that can be directly added to cell culture medium. These complexes fuse with the cell membrane and release DNA into the cytoplasm. The cells are transfected efficiently without cytotoxic effects. Use approximately 5-10 μg DOTAP per μg DNA and approximately 10-20 μg DOTAP per mL cell culture medium. The optimal working concentration and transfection time depends in part on the cell line used, and the type of material (RNA, DNA, protein) loaded.

Cationic liposome-forming compound for transfection of DNA, RNA and other negatively charged molecules into eukaryotic cells. Mixing DOTAP with DNA results in spontaneously formed stable complexes that can be directly added to cell culture medium. These complexes fuse with the cell membrane and release DNA into the cytoplasm. The cells are transfected efficiently without cytotoxic effects. Use approximately 5-10 μg DOTAP per μg DNA and approximately 10-20 μg DOTAP per mL cell culture medium. The optimal working concentration and transfection time depends in part on the cell line used, and the type of material (RNA, DNA, protein) loaded.

Suitable for transient and stable transfection of nucleic acids into primary neurons and cultured neuronal cell lines. Use approximately 15-120 mul Neuroporter(TM) Transfection Reagent and 6-8 mug DNA (in provided unique DNA Dilution buffer when required) per 6 cm cell culture plate. The following cells have been successfully transfected using the Neuroporter(TM) Transfection Kit: . C6 glioma (human). Cortical neurons (rat primary). Dorsal Root Ganglion (DRG) cells (rat). NT2 neurons(human precursor cells). NT neurons (human differentiated cells). Subventricular Zone (SVZ) cells (mouse). White matter cells (mouse)

适用于将核酸瞬时和稳定转染到培养的真核细胞中。 每 6 cm 细胞培养板使用约 4-16μL Escort IV 和 2μg DNA。方案优化提供了非常高效的转染。关于使用 Escort IV 成功转染的细胞列表，请参见 转染试剂选择指南 。

适用于瞬时和稳定地将DNA转染至培养的哺乳动物细胞中。 使用磷酸钙方法已成功转染了以下细胞：BAEC肠黑素瘤细胞CHO K1COS-7成纤维细胞（人胚胎、新皮肤）HEK293Huh7IMR-90LLC（Lewis肺癌）NIH3T3PC-12PCI-13SH-SY5YSK-HEP-1T47D

DOTAP (N-[1-(2,3-Dioleoyloxy)propyl]-N,N,N-trimethylammonium methyl-sulfate) 脂质体转染试剂是一种阳离子脂质DOTAP的脂质体配方。DOTAP可用于DNA的高效转染，包括酵母人工染色体（YAC）转染至真核细胞用于瞬时或稳定基因表达，并也适合于高效的将其他带负电分子，如RNA、寡核苷酸、和谷氨酸、核糖蛋白（RNP）复合体以及蛋白，转移至哺乳动物细胞的研究样本中。

20 µg 纯化的即用型的质粒DNA，更多可供20次转染Enables highly efficient DNA transfection in a variety of cell lines including CHO-K1, COS, LNCaP, NIH/3T3, 293, T24, C2C12, SF-9, primary human keratinocytes, primary aortic smooth muscle, primary rabbit myoblasts and human bone marrow endothelial cells (HBMEC)Recommended for use with CRISPR/Cas9 KO Plasmids, HDR Plasmids and Cre Vectorstore at 4° C; DO NOT FREEZE; protect from light

Exfect® Transfection Reagent 是一种基于生物可降解的高分子树枝状聚合物的转染试剂，适用于多种细胞的DNA 转染。由于所使用的活化树枝状聚合物具有均一的大小和确定的形状，因此可实现高重复性的转染结果。Exfect® Transfection Reagent 携带DNA 进入细胞后，可迅速释放DNA，并被快速降解，更大的降低了对细胞的毒性。转染试剂-DNA 复合物可以直接加入完全培养基中，血清和抗生素不影响其转染效果，转染前后都不需要更换培养基，操作十分简便。

Exfect® Transfection Reagent 是一种基于生物可降解的高分子树枝状聚合物的转染试剂，适用于多种细胞的DNA 转染。由于所使用的活化树枝状聚合物具有均一的大小和确定的形状，因此可实现高重复性的转染结果。Exfect® Transfection Reagent 携带DNA 进入细胞后，可迅速释放DNA，并被快速降解，更大的降低了对细胞的毒性。转染试剂-DNA 复合物可以直接加入完全培养基中，血清和抗生素不影响其转染效果，转染前后都不需要更换培养基，操作十分简便。

本制品专门为小鼠胚胎干细胞研发，是一种基于纳米材料的转染产品，实现了更低细胞毒性，并对以测试的大多数细胞系表现出高转染效率。

高度一致的pH值和盐浓度保证高度一致的转染效率，展示良好的实验重复性。

Xfect是一款高效更低毒的转染试剂，无需Opti-MEM，整个转染过程可兼容血清，适用于广泛细胞系类型。

Xfect是一款高效更低毒的转染试剂，无需Opti-MEM，整个转染过程可兼容血清，适用于广泛细胞系类型。

1 ml; 10mg/ml in sterile waterhighly efficient infection reagent used to introduce retroviral vectors into mammalian cellsalso known as hexamethrine bromide, 1,5-Dimethyl-1,5-diazaundecamethylene polymethobromidePolybrene® is a registered trademark of Abbott Laboratories Corp.Store at -20º C

20 mlReduced-serum medium suitable for transfections with DNA PlasmidsRecommended for use with Plasmid Transfection Reagent (sc-108061) and suspension of DNA for transfection including: shRNA Plasmids, CRISPR/Cas9 KO Plasmids, HDR Plasmids or Cre VectorModification of Eagle's Minimal Essential Medium, buffered with HEPES and sodium bicarbonate, and supplemented with hypoxanthine, thymidine, sodium pyruvate, L-glutamine, trace elements and growth factors; protein level is minimal with insulin and transferrin being the only protein supplements; phenol red included at a reduced concentration as a pH indicatorStore at 4° C; light sensitive

0.2 ml; Sufficient for 50-100 transfections (per well in a 6-well plate)Enables highly efficient DNA transfection in a variety of cell lines including CHO-K1, COS, LNCaP, NIH/3T3, 293, T24, C2C12, SF-9, primary human keratinocytes, primary aortic smooth muscle, primary rabbit myoblasts and human bone marrow endothelial cells (HBMEC)Recommended for use with shRNA PlasmidsEffective in both serum-containing medium and serum-free medium, offering high efficiencies with minimal cytotoxicitystore at 4° C; DO NOT FREEZE; protect from light

0.3 ml; sufficient for 50-100 transfections (using 12-well plates)enables highly efficient siRNA transfection in a variety of cell lines including HeLa, A549, Jurkat and NIH/3T3Effective in both serum-containing medium and serum-free medium, offering high efficiencies with minimal cytotoxicitystore at 4° C; do not freeze; protect from light

1.5 mlTRIS-EDTA based buffer prepared from RNase-free water suitable for storage and dilution of siRNApH 8store at 4° C

20 mlreduced-serum medium suitable for addition to siRNA suspension and siRNA transfection reagent, immediately prior to cell transfectionModification of Eagle's Minimal Essential Medium, buffered with HEPES and sodium bicarbonate, and supplemented with hypoxanthine, thymidine, sodium pyruvate, L-glutamine, trace elements and growth factors; protein level is minimal with insulin and transferrin being the only protein supplements; phenol red included at a reduced concentration as a pH indicatorstore at 4° C; light sensitive