Gateway™ LR Clonase™ II Enzyme mix

Name: Gateway™ LR Clonase™ II Enzyme mix
SKU: 11791100

Gateway™ LR Clonase™ II酵素ミックスは、エントリークローン（目的遺伝子の両末端にattL配列が付加されている）とデスティネーションベクター（attR配列を含む）の間でのin vitroの組換え反応を触媒し詳細を見る

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製品番号（カタログ番号）	数量
11791100	100反応
11791020	20反応

2 オプション

製品番号（カタログ番号） 11791100

価格（JPY）

281,000

Each

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数量:

100反応

Gateway™ LR Clonase™ II酵素ミックスは、エントリークローン（目的遺伝子の両末端にattL配列が付加されている）とデスティネーションベクター（attR配列を含む）の間でのin vitroの組換え反応を触媒し、発現クローンを作成します。Gateway™ LR Clonase™ IIには酵素とバッファーが一つのミックスに調整されており、少ないピペット操作で便利な10マイクロリットルの反応セットアップが可能です。

研究用にのみ使用できます。診断用には使用いただけません。

仕様

適合バッファー酵素バッファー

製品タイプLRクロナーゼ酵素ミックス

数量100反応

出荷条件ドライアイス

酵素LRクロナーゼ

製品ラインClonase, Gateway

Unit SizeEach

組成および保存条件

Gateway™ LR Clonase™ II酵素ミックスには、プロテイナーゼK溶液（2 μg/μL）とポジティブコントロールベクターが含まれます。-20℃または-80℃で保管してください。適切に保存した場合、6カ月間安定しています。

よくあるご質問（FAQ）

I performed an LR reaction and got high background after transformation. Can you please offer some troubleshooting tips?

– Check whether the reaction was transformed into an E.coli strain containing the F' episome and the ccdA gene – use an E.coli strain that does not contain the F&339; episome, e.g. OmniMAX 2-T1R, TOP10.
– Deletion (full or partial) of the ccdB gene – propagate in media with 50-100 mg/mL ampicillin and 15-30 µg/mL chloramphenicol.
– Contamination from another resistant strain.
– Check whether proper amount of DNA was used in the reaction.

I performed an LR reaction and got two distinct types of colonies (large and small) after transformation. What could be the possible reasons?

– Plasmid was lost during culture due to large size or toxicity – try incubating at 30 degrees C; use Stbl2 E.coli to stabilize the plasmid.
– Deletions (full or partial) or point mutations in the ccdB gene – obtain a new Destination vector.
– Small colonies may be unreacted entry clone that co-transforms with the Expression clone – reduce the amount of Entry clone to 50 ng per 10 µL reaction; reduce the volume of sample used for transformation to 1 µL; for a Destination vector with ampicillin selection marker, increase the ampicillin concentration to 300 µg/mL.

I performed an LR reaction and got no colonies after transformation, and the recombination positive control was not successful. Can you please offer some suggestions?

– Check the competent cells with pUC19 transformation.
– Increase the amount plated.

I performed an LR reaction and got few or no colonies after transformation, whereas the transformation control gave colonies. Can you please offer some suggestions?

– Increase the incubation time up to 18 hours.
– Make sure to treat reactions with proteinase K before transformation.
– Check whether the correct antibiotic was used for selection.
– Check whether the att site sequences are correct.
– Check whether the correct Clonase enzyme was used and whether it was functional.
– Check whether the recommended amount of DNA was used in the reaction.
– Perform the positive control recombination with pENTR-Gus plasmid.
– If the Entry clone or Destination vector is too large (>10 kb), incubate the LR reaction overnight, linearize the Destination vector or the Entry clone or relax the Destination vector with topoisomerase I.

Can I create a single Entry vector for use with DEST vectors that have N-terminal tags and C-terminal tags?

No, since a stop codon would be necessary for an N-terminal tagged destination vector, whereas the presence of a stop codon would block expression of the C-terminal tag.

View all Gateway™ LR Clonase™ II Enzyme mix, 100 Reactions FAQs