인용 및 참조 문헌 (1)

Invitrogen™

ViraPower™ Bsd Lentiviral Support Kit

ViraPower™ Bsd Lentiviral Support Kit에는 표적 유전자를 담은 바이러스 입자를 생성하기 위해 293FT 세포에 transfection하는 데 필요한 구성품이 들어있습니다. 이자세히 알아보기

카탈로그 번호	수량
K497000 K4970-00으로도 사용됨	20 reactions

카탈로그 번호 K497000

K4970-00으로도 사용됨

제품 가격(KRW)

2,166,000

20 reactions

제품 가격(KRW)

2,166,000

ViraPower™ Bsd Lentiviral Support Kit에는 표적 유전자를 담은 바이러스 입자를 생성하기 위해 293FT 세포에 transfection하는 데 필요한 구성품이 들어있습니다. 이 키트에는 ViraPower™ Lentiviral Packaging Mix, Lipofectamine™ 2000 Reagent, blasticidin이 들어있으며 안정한 선택을 위한 blasticidin 표지자를 갖는 ViraPower™ Lentiviral expression vector와 함께 사용하도록 만들어졌습니다. 이 키트는 ViraPower™ HiPerform™ Lentiviral vector를 포함해 본사의 모든 ViraPower™ Lentiviral vector에 사용할 수 있습니다.

Kit 구성:
• ViraPower™ Lentiviral Packaging Mix
• Lipofectamine™ 2000 (Cat # 11668027)
• Blasticidin powder (Cat # R21001)

연구용으로만 사용할 수 있습니다. 치료 또는 진단 목적으로 사용할 수 없습니다.

For Research Use Only. Not for use in diagnostic procedures.

배달 유형Lentiviral

용도(애플리케이션)Viral Expression

제품 유형Lentiviral Support Kit

수량20 reactions

벡터pLP

제품라인ViraPower

프로모터RSV, CMV

Unit SizeEach

구성 및 보관

Contents
The ViraPower™ Bsd Lentiviral Support Kit includes the following components:
• 195 μg of ViraPower™ Packaging Mix (Contains 195 μL of a mixture of pLP1, pLP2, and pLP⁄VSVG plasmids, at 1 μg⁄μL in TE Buffer, pH 8.0)
• 0.75 ml of Lipofectamine™ 2000 (Cat # 11668027)
• 50 mg of Blasticidin powder (Cat # R21001)

Storage
• ViraPower™ Packaging Mix: -20°C
• Lipofectamine™ 2000: +4°C (do not freeze)
• Blasticidin: -20°C

자주 묻는 질문(FAQ)

I used one of your lentiviral vectors but am observing cytotoxic effects after transduction. Can you please help?

Possible causes include:

- large volume of viral supernatant used for transduction
- cells sensitive to Polybrene regaent
- too much antibiotic used for selection
- antibiotic used too soon after tranduction
- gene of interest is toxic to cells

I transduced my lentiviral stock into my mammalian cell line but am getting poor expression of my gene of interest. What could have happened?

Poor expression could result from low transduction efficiency, too low of a MOI, too much antibiotic used for selection, usage of antibiotic too soon after transduction, harveting cells too soon after transduction, having a gene of interest that is toxic to cells, or rerrangement in the LTR regions of the expression construct plasmid DNA.

I transduced my lentiviral stock into my mammalian cell line but am getting no expression of my gene of interest. What could have gone wrong?

Here are some possible causes and solutions:
- Promoter silencing; CMV promoter is prone to silencing especially in mouse and rat cells, screen multiple antibiotic resistant clones and select the one with the highest expression levels
- Viral stocks stored incorrectly; aliquot and store at -80 degrees C, do not freeze/thaw more than 3 times

I prepared a lentiviral stock using one of your lentiviral vectors. I am trying to determine the titer using antibiotic selection but am not able to since the cells are very confluent and I am not getting antibiotic-resistant clones. Can you please offer some tips?

Here are some possible causes and solutions:

- Too little antibotic used for selection
- Selection performed on confluent cells; replate cells
- Viral supernatant not diluted sufficiently; titer lentivus using a wider range of 10-fold serial dilutions

I am using one of your lentiviral vectors and am getting a low lentiviral titer. Can you offer some troubleshooting tips?

Possible causes include:

- low transfection efficiency; Use a high-quality plasmid prep, 293FT cells under passage 16, ensure removal of Geneticin during transfection, ensure correct DNA:lipid ratio, and that cells are plated at the correct confluency
- transfected cells are not cultured in medium containing sodium pyruvate; this reagent provides an extra energy source for cells
- viral supernatant harvested too early; viral supernatants can generally be collected 48-72 hrs post-transfection
- viral supernatant too dilute; concentrate virus using CsCl purification
- viral supernatant frozen and thawed multiple times; 3 times should be the maximum freeze/thaw
- gene of interest is large; viral titers decrease as size of insert increases, inserts larger than 5.6 kb are not recommended
- rearrangement in the LTR region of the epxression construct plasmid DNA; use Stb3 cells for transformatin of the lentiviral construct
- poor choice of titering cell line; use HT1080 cells or similar cell line
- Polybrene reagent is not included during transduction; transduce lentiviral construct into cells in the presence of Polybrene reagent
- Lipofectamine reagent handled incorrectly; ensure proper storage and mix gently before use
- Use fluorescence micrscopy to check titer with HiPerform FastTiter lentivirus

Find additional tips, troubleshooting help, and resources within our Protein Expression Support Center.

View all ViraPower™ Bsd Lentiviral Support Kit FAQs

인용 및 참조 문헌 (1)

인용 및 참조 문헌

Abstract

P75 interacts with the Nogo receptor as a co-receptor for Nogo, MAG and OMgp.

Authors:Wang KC, Kim JA, Sivasankaran R, Segal R, He Z,

Journal:Nature

PubMed ID:12422217

In inhibiting neurite outgrowth, several myelin components, including the extracellular domain of Nogo-A (Nogo-66), oligodendrocyte myelin glycoprotein (OMgp) and myelin-associated glycoprotein (MAG), exert their effects through the same Nogo receptor (NgR). The glycosyl phosphatidylinositol (GPI)-anchored nature of NgR indicates the requirement for additional transmembrane protein(s) to transduce the inhibitory signals ... More