太鼎生物科技/太鼎食安科技

miRNA(microRNA) Expression &
Detection

miRNA表現與偵測套組-GFP系統

miRNA表現載體letimiRa－GFP

GFP miRNA Lentivirus/Vector (LentimiRa-GFP)

重組慢病毒表達載體(Lentiviral expression vectors); 具有高效率轉譯，及穩定插入基因之特點。因此，lentiviral 表現載體為miRNA delivery之主要工具。的交付使用最廣泛的運載工具。Abmgood提供全系列miRNA慢病毒表達載體（lentimira）。lenrimira具有會功能性之設計，包含CMV啟動子及GFP報導基因，另有定量好的病毒顆粒。每個miRNA Native Pri-miRNA之設計（〜400-500bp的），具有最佳之目標基因抑制效果。

Recombinant lentiviral expression vectors are the most widely used delivery vehicle for miRNA delivery due to their high efficiency transduction and stable integration. As a world leader in both lentiviruses and miRNA, ABM provides the most comprehensive selection of miRNA lentivirus expression vectors (lentimira). Each vector has been tested for functionality and contains a GFP reporter under a constitutive CMV promoter in both plasmid vector and ready-to-use viral particle formats. The design of native pri-miRNA (~400-500bp) for each miRNA offers higher levels of target gene suppression than those based on a single common miRNA backbone as seen with competitors. Please open the following (link or PDF file) for comparison.

Recombinant
lentiviral expression vectors are the most widely used delivery vehicle for
miRNA delivery due to their high efficiency transduction and stable
integration. As a world leader in both lentiviruses and miRNA, ABM provides the
most comprehensive selection of miRNA lentivirus expression vectors
(lentimira). Each vector has been tested for functionality and contains a GFP
reporter under a constitutive CMV promoter in both plasmid vector and
ready-to-use viral particle formats. The design of native pri-miRNA
(~400-500bp) for each miRNA offers higher levels of target gene suppression
than those based on a single common miRNA backbone as seen with competitors.
Please open the following (link or PDF file) for comparison.

Human GFP miRNA Lentivirus/Vector
(LentimiRa-GFP) Vector

Human GFP miRNA Lentivirus/Vector
(LentimiRa-GFP) Virus

LentimiRa-GFP-hsa-let-7a-1 Virus

miRNA ID	MI0000060
miRNA Name	hsa-let-7a-1
Accession No.	MI0000060
Genome Location	Chromosome 9:95978060:95978139 (+ Strand)
Species	Human
Insert Type	Pre-miRNA
Reporter	GFP
Vector Name	pLenti-III-mir-GFP
Vector Map
Viral Titer	107 pfu/ml

 

 

miRNA Lentivirus分析套組

Kits for miRNA Lentivirus Production

負責Sales: 許虹宜0920-312382

原廠網站: www.abmgood.com

公司網站: www.biopioneer.com.tw

Lenti病毒顆粒轉染試劑

Lentifectin™ Transfection Reagent

Lentifectin™
Transfection Reagents

Description	Lentifectin™ is a transfection reagent specially formulated with multiple cationic polymers for the production of Lentiviral vectors in vitro. It is shown that Lentiviral vectors produced with Lentifectin™consistently have higher titers than those produced with Calcium-phosphate transfection or with other types of lipid transfection reagents
Application	For production of high titer recombinant lentivirus plasmid in 293 cells.
Protocol
Image
Storage	Store at 4ºC. Do not freeze.
Notes	This product is distributed for laboratory research only. Caution: Not for diagnostic use .

負責Sales: 許虹宜0920-312382

原廠網站: www.abmgood.com

公司網站: www.biopioneer.com.tw

轉染試劑產品系列-RNAi專用轉染試劑

Transfection Reagents

RNAifectin™

1. 針對RNAi基因沉默表現，而設計的轉染試劑。

2. 有效轉染RNAi oligo's，於真核細胞表現。

3. 效能高，毒性弱。轉染RNAi之最佳選擇

負責Sales: 許虹宜0920-312382

原廠網站: www.abmgood.com

average M_n 258

CAS Number 26570-48-9

MDL number MFCD00081876

PubChem Substance ID 24871153

Properties

Related Categories	Acrylate, Homobifunctional PEGs, Materials Science, Poly(ethylene glycol) and Poly(ethylene oxide), Polymer ScienceMore...
mol wt	average Mn 258
contains	100 ppm MEHQ as inhibitor
refractive index	n 20/D 1.463
density	1.11 g/mL at 25 °C

Description

Packaging

100, 500 mL in glass btl

Price and Availability

SKU-Pack Size Availability Price (USD) Quantity

475629-100ML	Estimated Delivery 16.05.2012 - FROM Availability details for 475629-100ML Close Enter Quantity: Check Availability 1 Estimated Delivery from Schnelldorf 16.05.2012		40.40
475629-500ML	Estimated Delivery 16.05.2012 - FROM Availability details for 475629-500ML Close Enter Quantity: Check Availability 1 Estimated Delivery from Schnelldorf 16.05.2012		95.90

miRNA inhibitor雙雄

MicroRNA sponges: competitive inhibitors of small RNAs in mammalian cells

Abmgood生產長效型miRNA inhibitor，利用lentivirus 或是adenovirus 表現miRNA inhibitor，因其具有miRNA sponge的效果，可長期抑制內生性miRNA表現，效率更勝於市售的oligo-based miRNA inhibitor

高力價病毒 (107 pfu/ml, 2 x 50ul)濃縮液

高力價病毒純化套組

miRNA表現質體

更多miRNA相關產品請上abmgood  http://www.abmgood.com/

目前市面上不同miRNA inhibitor 其作用原理如下:

miRNA表現載體

產品特點:

1. 可插入基因組中,長期有效表現miRNA使用病毒濃縮液,感染率

2. 高搭配不同啟動子或是GFP標記,讓實驗設計更加靈活

3. 同步最新miRbase 版本

4. 提供千種以上miRNA表現質體提供貼心客製化服務,為你省時

高力價病毒 (107 pfu/ml, 2 x 50ul)濃縮液,純化套組

miRNA inhibitor

表現miRNA inhibitor,具有miRNA sponge的效果,可長期抑制內生性miRNA表現,不需長期購買oligo-based miRNA inhibitor

siRNA客製化病毒顆粒表現系統

RNAi並不一定有效，且其效能通常與siRNA的表現量息息相關。在早期的研究中，經常

發現僅有不到1%的轉殖植物可表現出基因靜默現象。Abmgood利用lentivector作為基因

呈遞的工具，有效且持久地提供siRNA的表現量。

To order individual product(s) check the corresponding box(es) on the right or to order a kit check the corresponding box on the bottom, and then click 'Add to Cart'.

siRNA客製化病毒顆粒

方便又省時 快速有效

不用自已養病毒、定量病毒。高力價siRNA Lenti病毒顆粒，直接感染細胞

【siRNA客製化病毒顆粒, 產品問與答】

1. 【問與答】慢病毒表現系統是依賴Tat或不依賴Tat ?

Tat-Independent.

2. 【問與答】如何知道陰性對照組是什麼?如何知道此對照組, 不會針對其它基因發生作用, 是否有任何標記?

It is specifically designed that it should bring down any gene based on sequence search. Using neomycin as your selection marker can show whether the negative control was successfully incorporated by the cell.

3. 【問與答】為何在感染iLenti-EGFP後, 細胞沒有表現EGFP螢光蛋白, 如此現像在在293T細胞株是有表現EGFP, 但是其它的細胞株則沒有表現EGFP蛋白?.

It is easy to see EGFP in 293 cells. Most of the other cell lines take about 48-73h to see the EGFP, and even then, the fluorescence activity may be low. The promoter strength for the EGFP gene varies with different cell line.
Refer to the paper "Transgenes Delivered by Lentiviral Vector are Suppressed in Human Embryonic Stem Cells in a Promoter-Dependent Manner" by Xia et al. in Stem Cells and Development 16:167-176 (2007).

EGFP expression is dependent on promoter strength, which may differ between different cell types. The promoter for the EGFP gene is from CMV. Even though the promoter is ubiquitous, the expression of EGFP may be suppressed in some target cells. That does not necessarily mean that the vector is not in the cells. The vector may be there and the siRNA may be expressed because the promoters for the siRNA are different.
You can try Western blotting against the target gene product along with a standard curve to evaluate whether siRNA is being expressed and functional in the target cells.

4. 【問與答】iLenti-system是第幾代?

It is third generation lentivirus.

5. 【問與答】What is our lentivirus based on?

Our system is based on inactivated HIV. All our packaging plasmids cannot be integrated into the host and they are transiently expressed only.

6. 【問與答】lentiviral vectors的3’ acceptor sites 功能是什麼?

It's for biosafety reason. The 5' splice donor and 3' acceptors sites enhance the biosafety of the vector by facilitating removal of the packaging sequence and RRE such that expression of the gene of interest in the transduced host cell is no longer Rev-dependent (Dull et al., 1998). It will inhibit viral production in stable cell lines.

7. 【問與答】如何確保 lentivirus 為replication-defective?

We cannot send a protocol for you to view but I can summarize what we do to ensure the virus' replication deficiency.

Lentiviral vector stocks are tested for the presence of replication-competent lentivirus (RCL) by monitoring p24 antigen expression in the culture medium of transduced 293T cells for 30 days. Serial passaging of the transduced p24 cells over this period allows for the amplification of RCL. Since the vectors are replication-defective, no amplification of p24 signal would normally be expected. However, if there were an increase in P24 signal over time, it would be indicative of RCL contamination. The p24 antigen is assayed with a commercial kit from http://www.zeptometrix.com/ . This assay has been performed on multiple vector lots without a positive result.

8. 【問與答】lentivirus transduction效能如何?

This depends on the cell line or type as each one is different. In general, the lentivirus is very efficient in most cell lines with 100% for 293 and other commonly used cells. The lowest efficiency observed is 10% and customers have to do evolution for a specific cell line using EGFP lentivirus. For customers that just need to generate a stable cell line, 1% trandsuction efficiency is enough as every transduced cell is permanently integrated with the vector. Therefore, 10ml of 10^6 cfu/ml would contain more than enough transduced cells.

I cannot open link for information on lentiviral particle production for generation of stable cell lines. Please send link.

Here is the link for iLenti lentivirus production for generation of stable cell lines:
http://www.abmgood.com/RNAex/pdfs/iLenti-siRNA%20Expression%20System.pdf

Click for Details          

 Kanamycin for bacterial selection and puromycin for mammalian selection. 

Click for Details  

 具有GFP reporterKanamycin for bacterial selection and puromycin for mammalian selection.

Custom siRNA Lentivirus (iLenti™) Services Agreement

siRNA客製化設計與合成服務同意書

 

Click to view.

 

PEG病毒濃縮產品，有效提高病毒力價。可應用於Lentivirus 病毒濃縮，提供病毒力價或環境sample病毒的濃縮.

PEG Virus Precipitation Kit (Biovision)
Catalog#: K904-200  | Size: 200 preparat

PEG病毒濃縮產品特點:

● 不須超高速離心

● 安全無毒性

● 可將病毒液濃縮10 至100 倍

● 適用於 Lentivirus、Retrovirus、等病毒。

● 包裝為5 倍無菌濃縮液，方便使用

 太鼎生物科技有限公司(02)86609496

業務專員 許 虹宜 0920312382

   As a world leader in lentiviral technology, ABM has developed a variety of different lentiviral expression systems which can be used to temporarily alter expression within a sample of cells or to moniter gene expression using reporter genes. These systems allow other scientists to produce their own lentiviruses.

Lentiviral 表現系統產品種類

Lentiviral Systems

Lentivirus Constitutive Vectors表現載體

Lentivirus CMV啟動子載體 

His Tag Lentiviral 載體 | HA Tag Lentiviral 載體 | HA-III Tag Lentiviral 載體

Lentivirus UbC, PGK or EF1α啟動子載體 

UbC Promoter Lentiviral載體 | PGK Promoter Lentiviral 載體 | EF1α Promoter Lentiviral 載體

Lentivirus 啟動子缺失載體

 Promoterless Lentiviral 載體 | Promoterless GFP Lentiviral 載體

Bicistronic/Tricistronic Lentiviral 載體

shRNA and miRNA Lentiviral 表現載體

RFP Fusion Tag Lentiviral 載體

綠螢光蛋白GFP Fusion Tag Lentiviral 載體

綠螢光蛋白GFP Bicistronic Lentiviral載體

Reporter Lentiviral 載體

Therapeutic Lentiviral 載體

Lentivirus 包裝系統

   As a world leader in lentiviral technology, ABM has developed two unique packaging mixtures. Each contains two or three plasmids to seperate the lentiviral structural and replication genes until time of viral production, and preventing the structural genes from being present in the packaged viral genome of the produced virus. This increases the safety for the user by making the produced viruses replication incompetent.

Products List

Lentiviral 包裝系統

產品介紹

  For the production of lentiviral particles, three components are generally required: 1) a lentiviral vector containing your inserts of interests (cDNA, shRNA, or miRNA), 2) one or two packaging vectors which contain all necessary viral structure proteins, 3) an envelope vector expressing Vesicular Stomatitis Virus (VSV) glycoprotein (G). The 3^rd(third) generation packaging system offers maximal biosafety as the lentiviral Rev gene is supplied as an independent vector from other structure genes, further eliminating the possibility of reverse recombinantion of vectors into a replication competent viral particles. The 3^rd(third) generation lentiviral packaging mix will only support lentiviral expression vector with a chimeric 5' LTR in which the HIV promoter is replaced with CMV or RSV, thus making it TAT-independent. Thus the 3^rd(third) generation lentiviral vectors will not support the production of 2^nd(second) generation lentiviral particle productions. All of the lentiviral vectors marketed by ABM are TAT-independent.

2^nd Generation Packaging Mix

3^rd Generation Packaging Mix

Lentivirus純化及定量套組

Lentivirus 純化 Kit

PuRetro™ Lentivirus Purification Kits產品特點

easy to use

very reliable

very affordable

Speedy Lentivirus 純化

Speedy Lentivirus 純化產品特點

  Recombinant lentiviral vectors have been shown to be a powerful tool for stable gene transfer to both dividing and non-dividing cells in vitro and in vivo.Through years of experience with lentiviral vectors, ABM has developed its own proprietary pLenti-combo packaging mix and an efficient protocol for rapid production of recombinant lentiviral vectors with titers up to 107IU/ml. The quickest and easiest way to purify and concentrate lentiviral particles up to 100x. The concentrated viral preparations can be used for in vivo injection or like applications that require high titer of viral particles.

ABM's Lentiviral表現載體產品特點

stable plasmid; rare plasmid DNA re-arrangement

very high yielding plasmid

no special competent cells required

His and HA tag compatible

ABM is THE source for your lentiviral expression needs!

Viral Stock Buffer Exchange Kit

Viral Stock Buffer Exchange Kit (Cat.# G130) is supplied separately from the recombinant viral purification kits. All recombinant viral purification kits do not contain the viral stock buffer exchange kit.
  The eluted recombinant virus is in a salt buffer but can be used directly for in vitro target cell transduction if the viral dilution is over 5X (i.e. 1.0μl of viral stock to 4μl culture medium). For higher titers of viral stock or viral dilutions less than 5X during transduction, a buffer exchange is required to make the viral stock suitable for such applications. This can be easily performed using ABM Inc.'s viral buffer exchange kit (Cat.# G130). The kit includes five exchange filters that are applicable for all recombinant viruses, as well as two specialized buffers, in sufficient quantities to run either five adenoviral or five lenti/retroviral or any combination of purifications.
Adenoviral storage buffer: 2.5% glycerol (w/v), 25mM NaCl, and 10mM Tris-HCl, pH 8.0 (Hoganson, et al., 2002).
Lentiviral/Retroviral storage buffer: 1X PBS buffer, pH at 7.2.

qPCR Lentivirus Titer (Titration) Kit

The Lentivirus Titration Kit provides a fast and simple method for titrating lentivirus. This kit employs a quick RNA extraction step and determines viral RNA using qRT-PCR. The whole assay could be completed in only 2 hours. The titer primers supplied in this kit are designed for all HIV-1 based vectors detection. With the help of the on-line titer calculator, titration of any lentiviral preparation could be easier than ever before.

ABM's Lentiviral qPCR Titer Kit病毒力價定量產品特點

no RNA purification -- saves time and eliminates inaccuracy

ready-to-use reagent mix -- reduces variability

qRT-PCR in one step -- more sensitive and accurate than other methods

no NTC amplification -- our titeration kit is the only one on the market that completely elimites NTC signal due to our unique primer design. Similar kits from other companies all give NTC amplification, which compromise accuracy for viral titeration

free qPCR mastermix -- a deal that can not be beat

詳細產品資訊，請登錄www.abmgood.com 查詢，或與太鼎生物科技有限公司(02)86609496聯繫。 

WWW.BIOPIONEER.COM.TW

太鼎生物科技有限公司(02)86609496

Lentivirus 純化產品. 其能有效增強病毒力價。

 Both recombinant retrovirus and lentivirus are widely used in the transduction of a varity of target cells and can be produced by transient transfection, from which viral supernatant can be collectedand used for target cell transduction. The titer of viral supernatant by transient transfection is approximately 10⁶ cfu (colony forming unit)/ml, which is sufficient Purification Experimental Flow Chart for the generation of most stable cell lines in vitro. However, there are applications that require higher purity and titers. These applications include experiments demanding higher gene transduction efficiency and in vivo gene delivery. In addition, crude viral supernatants are not suitable for in vivo administration due to various contaminants contained in cell culture supernatant. Thus, the viral supernatant needs to be further concentrated and purified before use.
  Traditionally, both recombinant retrovirus and lentivirus have been concentrated via ultracentrifugation. Although the method works well, it requires specific ultracentrifugation equipment and it is technically demanding. In addition, the total viral supernatant volume is limited to the size of ultracentrifugation tubes. Reports have also stated that the ultracentrifugation process has some detrimental physical effects on the recombinant virus.
  Due to limitations on the existing technique, there is great necessity for a quick and efficient method to purify and concentrate recombinant retrovirus and lentivirus. Scientists at ABM Inc. have had years of experience with Ion-Exchange-based filter membranes and have successfully developed PuRetro™, the most effective retroviral and lentiviral purification method based on this technology.

Advantages of PuRetro™ Lentivirus Purification Kits

·        easy to use

·        very reliable

·        very affordable

【太鼎生物科技有限公司02-86609496】ABMGOOD台灣總代理

Citations

1.    Buchschacher, G. L., Jr., and Wong-Staal, F. (2000) Development of Lentiviral Vectors for Gene Therapy for Human Diseases. Blood 95, 2499-2504.

2.    Burns, J. C., Friedmann, T., Driever, W., Burrascano, M., and Yee, J.-K. (1993) Vesicular Stomatitis Virus G Pseudotyped Retroviral Vectors: Concentration to a Very High Titer and Efficient Gene Transfer into Mammalian and Nonmammalian Cells. Proc. Natl. Acad. Sci. USA 90, 8033-8037.

3.    Demmer, W. and Nussbaumer, D. 1999. Large-scale Membrane Adsorbers. J. Chromatogr. A., 852:73-81.

4.    Dull, T., Zufferey, R., Kelly, M., Mandel, R. J., Nguyen, M., Trono, D., and Naldini, L. (1998) A Third-Generation Lentivirus Vector with a Conditional Packaging System. J. Virol. 72, 8463-8471.

5.    Graham, R.L., Smiley, J., Russel, W.C., and Narin, R. 1977. Characteristics of a human cell line transformed by DNA from human adenovirus type 5. J. Gen. Virol., 36:59-72.

6.    Hoganson, D.K., Ma, J.C., Asato, L., Ong, M., Printz, M.A., Huyghe, B.G., Sosnowshi, B.A. and D'Andrea, M.J. 2002. Development of a stable adenoviral vector formulation. Bioprocessing J. 1(1):43-48.

7.    Hutchins, B. 2002. Development of a reference material for characterizing adenovirus vectors. Bioprocessing J., 1(1):25-28.

8.    Lochmuller, H., Jani, A., Huard, J., Prescott, S., Simoneau, M., Massie, B., Karpati, G., and Acsadi, G. (1994). Emergence of Early Region 1-Containing Replication-Competent Adenovirus in Stocks of Replication-Defective Adenovirus Recombinants (Delta E1 + Delta E3) During Multiple Passages in 293 Cells. Hum. Gene Ther. 5, 1485-1491.

9.    Wang, I. I. , and Huang, I. I. (2000). Adenovirus Technology for Gene Manipulation and Functional Studies. Drug Discovery Today 5, 10-16.

10. Wivel, N. A. (1999) Adenoviral Vectors. In The Development of Human Gene Therapy, T. Friedmann, ed.( Cold Spring Harbor , NY : Cold Spring Harbor Laboratory Press), pp. 87-110.

11. Yamada, K., McCarty, D.M., Madden, V.J., and Walsh, C.E. (2003). Lentivirus Vector Purification Using Anion Exchange HPLC Leads to Improved Gene Transfer. Biotechniques 34:1074-1080.

What is the difference between Retro-, Lenti-, and Adeno- viruses?

Retrovirus: Classic, can integrate into the genome but with low transduction efficiency. They are useful for gene transfer and protein expression in cells that have low transfection efficiency with other transfection reagents.

Lentivirus: Can integrate into the genome with relatively high transduction efficiency and they are very useful for cells that have low transfection efficiency with other transfection reagents. No special competent cells required, as they are stable plasmids. Lentiviruses are a powerful tool for stable gene transfer to both dividing and non-dividing cells in vitro and in vivo.

Adenovirus: Only work transiently (about 7 days) but have almost 100% transduction efficiency. Adenoviruses can infect a broad range of cell types with the highest efficiency and infection is not dependent on active host cell division. A second key feature is that high virus titers and high-level gene expression can be obtained in most mammalian cells.

What are the correct concentration units for each recombinant viral particle?

For lentiviruses and retroviruses, they are measured in CFU/ml (colony-forming units per millilitre). Transduction with lentiviruses and retroviruses can cause the formation of colonies, which can be quantified for concentration. Adenoviruses are measured as PFU/ml (plaque-forming units per millilitre). Transduction with adenoviruses will kill packaging cells, forming plaques in the process for quantification. The concentration for all three types of viruses can also be classified as IU/ml (Infectious Units/ml). Ultimately, the units refers to the viral particles and different units reflect the different assays involved.

Both recombinant retrovirus and lentivirus are widely used in the transduction of a varity of target cells and can be produced by transient transfection, from which viral supernatant can be collectedand used for target cell transduction. The titer of viral supernatant by transient transfection is approximately 10⁶ cfu (colony forming unit)/ml, which is sufficient Purification Experimental Flow Chart for the generation of most stable cell lines in vitro. However, there are applications that require higher purity and titers. These applications include experiments demanding higher gene transduction efficiency and in vivo gene delivery. In addition, crude viral supernatants are not suitable for in vivo administration due to various contaminants contained in cell culture supernatant. Thus, the viral supernatant needs to be further concentrated and purified before use.
  Traditionally, both recombinant retrovirus and lentivirus have been concentrated via ultracentrifugation. Although the method works well, it requires specific ultracentrifugation equipment and it is technically demanding. In addition, the total viral supernatant volume is limited to the size of ultracentrifugation tubes. Reports have also stated that the ultracentrifugation process has some detrimental physical effects on the recombinant virus.
  Due to limitations on the existing technique, there is great necessity for a quick and efficient method to purify and concentrate recombinant retrovirus and lentivirus. Scientists at ABM Inc. have had years of experience with Ion-Exchange-based filter membranes and have successfully developed PuRetro™, the most effective retroviral and lentiviral purification method based on this technology.

Advantages of PuRetro™ Lentivirus Purification Kits

·        easy to use

·        very reliable

·        very affordable