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icon below as well as clone information before placing your order.
pAxCALNLEGFP (forward) (#RDB03259)
Shuttle vector for rAd harboring enhanced green fluorescent protein cDNA.
| Alternative name | 625C1 |
|---|---|
| Clone info. | Enhanced green fluorescent protein (EGFP) is cloned into the SwaI site of pAxCALNLw. (Direction:forward) |
| Comment | Cre-recombinase is required to remove LNL stuffer sequence. Use COS-TPC method for the production of adenovirus. |
| Vector backbone | pAxCALNLw (Cosmid, use packaging extracts for transforming E. coli host) |
| Size of vector backbone | 45,995 bp |
| Selectable markers | Amp^r |
| Gene/insert name | Aequorea victoria GFP cDNA |
| Depositor|Developer | DNA Bank, | |
Distribution information
Please check terms and conditions set forth by the depositor, which are specified in the RIKEN BRC Catalog and/or Web Catalog.
| Ordering forms | Order form [Credit Card Payment  ] [Bank Transfer Payment] [Example of order form ]MTA, for use for not-for-profit academic purpose [Word ] [Example of MTA ]Please visit Information of Request for Distribution.[link] |
|---|---|
| Terms and conditions for distribution | 1. The RECIPIENT agrees to use the BIOLOGICAL RESOURCE only for academic research in the non-profit organization. 2. In publishing the research results to be obtained by use of the BIOLOGICAL RESOURCE, an acknowledgment to the DEPOSITOR is requested. Additional terms and conditions: Regarding resources containing CAG promoter: In publishing the research results obtained by use of the BIOLOGICAL RESOURCE, a citation for the CAG promoter (Niwa, H., Yamamura, K., Miyazaki, J., Gene 108 : 193-200, 1991) and an acknowledgment to Dr. Jun-ich Miyazaki of the Osaka University are requested. |
| Remarks | Remember that you will be working with samples containing infectious virus. |
[open/close]| 必要書類 | 提供依頼書 [依頼書の記入例 ]提供同意書 (MTA, 非営利学術目的用)[Word ] [MTAの記入例 ]手続きの概要は、「提供申込みについて[link]」をご覧ください。 |
|---|---|
| MTAに書く使用条件 | 1. 本件リソースは非営利機関にのみ提供し、学術研究にのみ利用することができる。 2. 謝辞の表明を必要とする。 MTAに書く付加的使用条件: CAGプロモータを含むリソースについて: 利用者は、研究成果の公表にあたってCAGプロモータの文献 (Niwa, H., Yamamura, K., Miyazaki, J., Gene 108 : 193-200, 1991)を引用し、大阪大学 宮崎純一博士への謝辞の表明を必要とする。 |
| 備考 | このリソースはウイルス粒子産生用のため、取扱いに注意が必要です。 |
| Catalog # | Resource name | Availability | Shipping form | Fee (non-profit org.) |
|---|---|---|---|---|
| RDB03259 | pAxCALNLEGFP (forward) | Under QC test. Please contact us. | DNA solution |
Please wait for results of QC test to be uploaded. This clone will be sequenced a portion for examination.How to cite this biological resource
Materials & Methods section:
| The pAxCALNLEGFP (forward) was provided by the RIKEN BRC through the National BioResource Project of the MEXT, Japan (cat. RDB03259). |
Reference section:
Further references such as user reports and related articles (go to bottom)
QC test results
Please wait for results of QC test to be uploaded. This clone will be sequenced a portion for examination.
References
Original, user report and related articles
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Aequorea victoria GFP
Reference sequence
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