Celthy脂质体转染试剂,增强研究人员对转染成功的信心-商家动态-资讯-生物在线

Celthy脂质体转染试剂,增强研究人员对转染成功的信心

作者:上海魔兜儿生物科技有限公司 2024-12-13T00:00 (访问量:2442)

背景介绍

转染使我们能够更好地理解目标基因在细胞中是如何表达和调节的。目前常见的转染方法包括磷酸钙共沉淀、电穿孔、DEAE-葡聚糖和聚脲嘧啶、机械方法(如显微注射和基因枪)以及阳离子脂质体转染试剂,其中阳离子脂质体转染试剂是常用的一种。

Figure 1: Schematic Diagram of Different Transfection Methods (Image source: Daily Biology Reviews)

 

不同转染方法比较

Transfection Method

Advantages

Disadvantages

Calcium Phosphate Co-precipitation

Low cost, relatively simple operation 

Unstable transfection efficiency, prone to issues such as DNA aggregation affecting transfection efficiency, high cytotoxicity, poor transfection efficiency

Electroporation

High efficiency, suitable for all types of cells

Expensive electroporation equipment, high cell death rate, requires large amounts of nucleic acids and cells

DEAE-Dextran

Effective for transfection of adherent cells, can also be used for certain suspension cells, simple operation, repeatable results

Cell preference, some toxicity to cells, serum inhibition of cell growth required during transfection

Polybrene

Relatively simple operation, moderate price

Low efficiency, some limitations in application

Cationic Lipid Reagents

Simple operation, high efficiency, wide applicability, good repeatability, low toxicity

Slightly higher price compared to other chemical reagents

Viral Transduction

High efficiency, effective for difficult-to-transfect cells, good transduction in primary cells

Complex viral packaging process, some risk associated with viruses

Polyethylenimine (PEI)

Low price, simple operation, wide applicability

Lower efficiency compared to lipid-based transfection reagents, some cells exhibit sensitive reactions after contact

 

已验证细胞系

Celthy Trans脂质体核酸转染试剂作为一种阳离子脂质体转染试剂,与广泛使用的Lipo2000相比,具有更高的转染效率和更便捷的操作性。它已在多种细胞系中得到验证,如下是经过验证的细胞系列表。

A549

BV-2

BV50

C2C12

Calu 1

CHO

Caco2

C6

COS-7

DF-1

H299

H520

HaCaT

HCT116

HEK293

HEK 293T

HeLa

Hep2C

Hep3B

Hepa1-6

HepG2

HK2

HO1980

HUVEC

HaCaT

HUVEC

H520

H9C2

H9

LM3

Lenti X-293T

MCF10A

MCF-7

MDA-MB-231

MDCK

MEF

MKN-28

N2A

NCI-H1975

NIH-3T3

Neuro-2a

PC12

Raw264.7

RKO

SGC-7901

SMCC7721

T47D

THP-1

TS

U-87

Vero

WEHI

WRL-68

3t3

5-8F

93T

293FT

多发性骨髓瘤细胞

More…

 

 

 

 

 

作用机理

阳离子脂质体可以通过其表面的正电荷与核酸的负电荷通过静电相互作用包裹核酸,形成核酸-脂质体复合物。细胞膜表面带有负电荷,使得复合物能够被吸附。一旦被吸附,复合物可以通过膜融合或内吞作用进入细胞,形成细胞内的包含体。一小部分DNA可以从包含体中释放出来,进入细胞质,进一步进入细胞核进行转录和表达。

Figure 2: Liposome-mediated Transfection and Endocytosis Process

 

转染试剂产品特点:

高效率:能够转染大多数真核细胞,对常见细胞系的转染效率超过90%;

低毒性:转染的细胞形态良好,能高水平表达转染的基因蛋白;

操作便捷:脂质体复合物可以直接添加到含有血清的培养基中;

多用途:适用于瞬时和稳定转染实验。

 

操作流程

Figure 3: Cell Transfection Experimental Workflow

 

产品数据

Figure 4: Dual Plasmid Transfection Reagent Validation Results

 

客户反馈数据

Celthy Trans Liposomal Transfection Application

Activation of Cell Autophagosome Formation by Bacterial Protein

Cell: HeLa

Transfected Plasmid: Bacterial Effector Protein A

LC3II: Autophagosome Marker Protein

Hoechst 33342 Spindle Structure during Cell Division

Cell: HeLa

Transfected Plasmid: Flag-tubulin

Nuclear Staining: Hoechst 33342

Celthy Trans

Lipo3000

 Celthy Trans

Lipo2000

Image Source: Fudan University

Cell Line: HEK293

Nucleic Acid Type: DNA

Image Source: Changchun Institute of Applied Chemistry

Cell Line: HeLa

Nucleic Acid Type: DNA

Flow Cytometry Fluorescence Observation Results

Celthy Trans (13.27%)

Lipo2000 (8.64%)

FuGenHD (9.24%)

Cell Line: C2C12

Fluorescent Protein: EGFP (Enhanced Green Fluorescent Protein)

Nucleic Acid Type: DNA

Data Source: South China Agricultural University

 

客户提供的部分细胞转染数据(仅供参考)

Cell

Culture Plate

Cell Density

DNA

Celthy Trans

Efficiency

293T

6 well

80%

1μg

2μL

90%

293FT

24 well

85%

1μg

4μL

90%

Hela

12 well

90%

0.2μg

0.6μL

90%

Raw264.7

35mm plate

80%

1μg

2μL

90%

Hek293

6 well

95%

2μg

10μL

80-90%

NCI-H1975

6 well

80%

4μg

10μL

80%

3t3

12 well

90%

1μg

5μL

50%

 

常见问题

Q1: 准备核酸转染试剂复合物时可以有血清存在吗?

a: 血清的存在可能会影响脂质体的形成。建议在准备核酸转染试剂复合物时使用无血清培养基(通常为MEM培养基)。

Q2: 在转染实验中需要更换为无血清培养基吗?

a: 不需要,我们的转染试剂可以在含有血清的培养基中进行转染。

Q3: 转染后需要终止转染吗?

a: 不需要。脂质体复合物可以稳定存在6小时。如果转染前没有更换细胞培养基,需要在转染后4-6小时更换为新鲜培养基,以确保细胞正常生长所需的营养物质。但如果转染前已经更换了培养基,则在脂质体转染后不需要再次更换培养基。

Q4: 存储和使用转染试剂时需要注意什么?

a: 该试剂必须存放在4°C。避免反复长时间开盖,因为长时间暴露在空气中可能会导致脂质体氧化,影响转染效率。

Q5: 如何提高转染效率?

a: 转染时的细胞密度,保持在90%-95%。

b: 转染过程中使用MEM无血清培养基稀释核酸和脂质体稀释液。

c: 转染后4-6小时可以更换培养基。

 

产品推荐

Product Name

Catalog number

Specification

Celthy Univer Liposomal Transfection Reagent 

C130002S

0.5 mL

C130002M

1.0 mL

 

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