JP7364331B2 - パエニバチルス(Paenibacillus)属種マンナナーゼ - Google Patents
パエニバチルス(Paenibacillus)属種マンナナーゼ Download PDFInfo
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- JP7364331B2 JP7364331B2 JP2018522994A JP2018522994A JP7364331B2 JP 7364331 B2 JP7364331 B2 JP 7364331B2 JP 2018522994 A JP2018522994 A JP 2018522994A JP 2018522994 A JP2018522994 A JP 2018522994A JP 7364331 B2 JP7364331 B2 JP 7364331B2
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- mannanase
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Description
本出願は、2015年11月5日出願の米国仮特許出願第62/251516号明細書、及び2016年1月13日出願の米国仮特許出願第62/278387号明細書の優先権の利益に関し、且つこれを主張する。これらの出願は双方とも、それらの全体が参照によって本明細書に組み込まれる。
ASCIIテキストファイル(名前:NB40843WOPCT_ST25;サイズ:321KB;作成日:2016年11月3日)として本出願と共に電子的に提出された配列表の内容は、本出願の一部を形成し、そしてその全体が参照によって本明細書に組み込まれる。
パエニバチルス(Paenibacillus)属種マンナナーゼPspMan138のクローニング及び発現
パエニバチルス属(Paenibacillus)種PspMan4マンナナーゼ変異体PspMan138を生じさせるDNA操作を、従来の分子生物学技術を用いて実行した(例えば、Sambrook et al,Molecular Cloning:Cold Spring Harbor Laboratory Press参照)。野生型パエニバチルス(Paenibacillus)属種PspMan4マンナナーゼの配列中に複数のアミノ酸改変を導入した人工DNA配列を生じさせた。当該野生型マンナナーゼは、2015年7月10日出願の国際出願PCT/US15/40057号明細書(後に国際公開第2016/007929号パンフレットとして公開)中により完全に記載されている。
マンナナーゼの活性及び安定性を特徴付ける方法
生化学的特徴付け用にPspMan4(成熟したタンパク質のアミノ酸配列を、配列番号14として示す)及びPspMan138変異体(配列番号13)の酵素サンプルを作製するために、形質転換した枯草菌(B.subtilis)細胞の選択的増殖を、96ウェルマイクロタイタープレート(MTP)中で37℃にて68時間、各ウェル内の培地(主要な窒素源としての尿素、主要な炭素源としてのグルコースを有し、ロバストな細胞増殖のために1%ソイトンを補った、MOPSバッファに基づく半規定富化培地)中で実行した。培養物を、3600rpmにて45分間の遠心分離によって収穫して、Multiscreen(登録商標)フィルタプレート(EMD Millipore,Billerica,MA,USA)により、Millipore真空系を用いて濾過した。濾過した培養液の上澄みを、以下に記載するアッセイに用いた。
PspMan4及びそのPspMan138変異体のマンナナーゼ活性を、溶液中ローカストビーンガム(LBG)ガラクトマンナンの加水分解を測定することによって試験した。用いた基質は、50mMトリスHClバッファ、pH7.5(基質希釈バッファ)中0.28%(w/v)LBG溶液であった。作用基質溶液を調製するために、LBG粉末(製品No.G0753,Sigma-Aldrich,St.Louis,MO)を、50mMトリスHClバッファ、pH7.5の加熱溶液中に撹拌下で溶解させた。室温に冷却して直ぐに、溶液を遠心分離して、澄明な上澄みを基質溶液として用いた。酵素サンプルを、酵素希釈バッファ(50mM MOPSバッファ、pH7.2、0.005%TWEEN(登録商標)-80含有)中に希釈して、希釈した酵素溶液のアリコートを、LBG基質溶液を含有する平底クリアポリスチレンMTPに加えた。プレートをシールして、900rpmでの撹拌(例えばiEMSインキュベーター/シェーカー、Thermo Fisher Scientific,Waltham,MA)により40℃にて10分間、インキュベートした。インキュベーションの後、放出された還元糖を、BCA試薬アッセイ(カタログNo.23225、Thermo Scientific Pierce,Rockford,IL)を用いて定量化した。詳細には、LBGアッセイプレートの各ウェル由来のアリコートを、BCA作用試薬溶液(メーカーの説明書に従って調製した)を含有するPCRプレートに加えた;サンプル対作用試薬の比は、1:9(v/v)であった。プレートをシールして、サーモサイクラー(例えばTetrad2 Peltier Thermal Cycler,Bio-Rad Laboratories,Hercules,CA)内で95℃にて2~3分間インキュベートした。プレートを30℃に冷却した後、反応溶液を、フレッシュな平底クリアポリスチレンMTP(例えばCostar 9017)に移して、吸光度をプレートリーダー分光光度計(例えばSpectraMax Plus 384,Molecular Devices,Sunnyvale,CA)内で562nmにて測定した。マンナナーゼを含有しないサンプル(ブランク)の吸光度の値を、マンナナーゼ含有サンプルの吸光度の値から減算した。生じた吸光度を、マンナナーゼ活性の尺度とした。
PspMan4及びそのPspMan138変異体の安定性を、ストレス条件下で、市販のTIDE(登録商標)液体洗濯洗剤(Original scent,Procter and Gamble、2014年に一地方のスーパーマーケットで購入して、以下の実施例4に記載するプロトコルを用いて熱不活化した)の10%(v/v)水溶液中で、高温(56℃)にて5分間インキュベーションした後のサンプルの残留活性を測定することによって、試験した。
マンナナーゼの洗浄性能
マンナナーゼ酵素を、MESバッファpH5.3中での硫酸アンモニウム沈殿によって清澄化したバチルス(Bacillus)属培養液の上澄みから単離した。精製を、疎水性交換クロマトグラフィに続く、50mM MESバッファ、pH6.0中への透析によって達成した。次に、プロピレングリコールを加えて40%の最終濃度にして、サンプルを、更なる特徴付けまで冷蔵保存した。
市販の液体洗濯洗剤中でのマンナナーゼの半減期の判定
市販の洗剤の不活化
本明細書中で以下に示す表3に一覧にする液体洗濯洗剤を、一地方のスーパーマーケットで購入した。バックグラウンド酵素活性を無効にするために、これらの市販の洗剤中に存在する酵素を、洗剤を95℃にて3~4時間の加熱することによって、不活化した。加熱後、洗剤を、本明細書中で以下に示すプロテアーゼ及びアミラーゼ活性アッセイを介して、酵素活性についてアッセイした。洗剤を4時間加熱した後、プロテアーゼ及びアミラーゼ活性は、検出されなかった。さらに、熱不活化洗剤中のマンナナーゼ活性の不在が、以下の「残留マンナナーゼ活性アッセイ」中で記載するLBG基質に対する活性アッセイによって示された。
最初に洗剤を50mM MOPSバッファ、pH7.2中に1:5で希釈することによって、酵素活性を測定した。
マンナナーゼのβ-1,4-マンナナーゼ活性を、放出された還元糖を定量化することによって測定した。用いた基質は、0.28%LBGガラクトマンナン(Sigma G0753)であった。放出された糖を、還元糖と反応するジニトロサリチル酸(DNS)を用いて定量化した;その540nmでの吸光度は、酵素活性と比例する。
相同マンナナーゼの同定
関連タンパク質を、PspMan138の成熟したアミノ酸配列(配列番号13)を用いて、NCBI非重複タンパク質データベースに対するBLAST検索(Altschul et al.,Nucleic Acids Res,25:3389-402,1997)によって同定した。サブセットを表5Aに示す。類似した検索を、Genome Quest Patentデータベースに対してランした。検索パラメータは、PspMan138の成熟したタンパク質アミノ酸配列(配列番号13)をクエリ配列として用いるデフォルト値に設定した。サブセットを表5Bに示す。
PspMan138(配列番号13)及び親PspMan4(配列番号14)を含むNDL-クレードマンナナーゼについての成熟したタンパク質アミノ酸配列の、BciMan1_BAA25878.1(配列番号40)、バチルス(Bac.)属種_BAD99527.1(配列番号43)、B.ネアルソニィ(B_nealsonii)_AGU71466.1(配列番号42)、バチルス(Bac.)属種_WO2015022428-0015(配列番号44)、B.レンタス(B.lentus)_WO2014100018-0002(配列番号41)、US6566114-002(配列番号160)、並びにPamMan2、PamMan3、PtuMan2、PpaMan2、及びPspMan9(これらは、2015年7月10日出願の国際特許出願PCT/US15/40057号明細書(後に国際公開第2016/007929号パンフレットとして公開)においてより完全に記載されている)の成熟した形態を含む他のマンナナーゼの成熟したタンパク質アミノ酸配列とのアラインメントを、図2に示す。配列を、Geneiousソフトウェア(Biomatters Ltd.)のMUSCLEプログラム(Robert C.Edgar.MUSCLE:multiple sequence alignment with high accuracy and high throughput Nucl.Acids Res.(2004)32(5):1792-1797)を用いて、デフォルトのパラメータでアラインした。図2の種々のマンナナーゼの成熟した形態のアミノ酸配列についての系統樹を、Geneious Treeビルダープログラムを用いて構築して、図3に表す。
PspMan138マンナナーゼの特有の特徴
PspMan138(配列番号13)及び親PspMan4(配列番号14)のアミノ酸配列を、CLUSTALWソフトウェア(Thompson et al.,Nucleic Acids Research,22:4673-4680,1994)を用いて、デフォルトのパラメータでアラインして、図2に示した。アラインメントは、PspMan138及びPspMan4が、残基Trp31からIle40まで延びるモチーフを共有していることを示した。ポリペプチドのアミノ酸位置は、配列番号14に示すアミノ配列との対応によって番号を付けている。NDLマンナナーゼは、クレード(以降NDL-Cladeと呼ぶ)を生じさせる特徴を共有しており、用語NDLは、N末端近くの保存された残基NDL(Asn34-Asp35-Leu36)に由来する。このモチーフを、WXaKNDLXXAI(配列番号15)と記載することができ、式中、Xaは、F又はYであり、Xは、あらゆるアミノ酸である(「モチーフ1」)。当該モチーフは、2015年7月10日出願の国際特許出願PCT/US15/40057号明細書(後に国際公開第2016/007929号パンフレットとして公開)においてより完全に記載されている。
付加的なパエニバチルス(Paenibacillus)属種PspMan4変異体のクローニング及び発現
付加的なパエニバチルス(Paenibacillus)属種PspMan4変異体を生じさせるDNA操作を、実施例1に記載するようにして、表1に一覧にしたプライマーで実行した。親PspMan4(配列番号14)に対して配列置換が生じたPspMan4変異体のリストを、表6に示す。成熟したPspMan4変異体のアミノ酸配列:PspMan115~122、PspMan124~130、PspMan132~145、PspMan148、PspMan150~158、PspMan6153、PspMan6428、PspMan6435、PspMan6574、PspMan6668、PspMan6670、PspMan6722、PspMan7154、PspMan_HM48~64、PspMan_HM66~67、及びPspMan_HM71を、配列番号46~91、141~159、及び161に示す。
ミクロスワッチアッセイを用いたPspMan4変異体の洗浄性能
生化学的特徴付け用にPspMan4変異体酵素サンプルを作製するために、形質転換した枯草菌(B.subtilis)細胞の選択的増殖を、96ウェルMTP中で37℃にて68時間、各ウェル内の培地(主要な窒素源としての尿素、主要な炭素源としてのグルコースを有し、ロバストな細胞増殖のために1%ソイトンを補った、MOPSバッファに基づく半規定富化培地)中で実行した。培養物を、3600rpmにて45分間の遠心分離によって収穫して、Multiscreen(登録商標)フィルタプレート(EMD Millipore,Billerica,MA,USA)により、Millipore真空系を用いて濾過した。濾過した培養液の上澄みを、以下に記載するアッセイに用いた。
バッファ溶液中でのPspMan4変異体の安定性
高温にて5分間のインキュベーション後にサンプルの残留活性を測定することによって、PspMan4変異体の安定性を、表8に示す温度での、50mM MOPSバッファ、pH7.2、0.005%TWEEN(登録商標)-80におけるストレス条件下で試験した。バッファ中でのタンパク質安定性アッセイに用いた条件を、表8に示す。
先に記載したように、ストレスを受けた活性の値及びストレスのない活性の値を、LBG基質の加水分解によって一旦測定して、ストレスを受けた活性の、ストレスのない活性に対する比率をとって、100を乗じることによって、%残留活性を算出した。表9は、表8に記載した条件下での安定性アッセイにおいて、PspMan4親よりも安定性が向上したPspMan4変異体を示す。
洗剤溶液中でのPspMan4変異体の安定性
PspMan4変異体の安定性を、ストレス条件下で、市販のTIDE(登録商標)液体洗濯洗剤(Original scent,Procter and Gamble、2014年に一地方のスーパーマーケットで購入して、実施例4に記載したプロトコルを用いて熱不活化した)の10%(v/v)水溶液中で、高温(表10に示す)にて5分間インキュベーションした後のサンプルの残留活性を測定することによって、試験した。
先に記載したように、ストレスを受けた活性の値及びストレスのない活性の値を、LBG基質の加水分解によって一旦測定して、ストレスを受けた活性の、ストレスのない活性に対する比率をとって、100を乗じることによって、%残留活性を算出した。誤差限界は、約5%以内であった。表11は、表10に記載した条件下での安定性アッセイにおいて、PspMan4親よりも安定性が向上したPspMan4変異体を示す。
Terg-o-tometer中でのPspMan118変異体の洗浄性能
PspMan118を、MESバッファpH5.3中での硫酸アンモニウム沈殿によって清澄化したバチルス(Bacillus)属培養液の上澄みから単離した。精製を、疎水性交換クロマトグラフィに続く、50mM MESバッファ、pH6.0中への透析によって達成した。次に、プロピレングリコールを加えて40%の最終濃度にして、サンプルを、更なる特徴付けまで冷蔵保存した。
PspMan4変異体の結晶構造
PspMan4変異体、PspMan118及びPspMan148の三次元構造を、X線結晶学的方法を用いて判定した。
PspMan4変異体の、年数を経た洗浄性能
PspMan4変異体を、100%洗剤中での室温でのインキュベーションの前後の洗浄性能について試験した。インキュベーション後の残りの%洗浄活性を、インキュベーション前の初期の洗浄活性と比較した。
Claims (16)
- 配列番号14のアミノ酸配列を有する基準ポリペプチドに由来し、マンナナーゼ活性を有する、マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片であって、
前記基準ポリペプチドと比較した改変として以下のアミノ酸置換の組み合わせまたはアミノ酸置換の組み合わせおよび位置298でのQの挿入(以下、「Z298.01Q」という。):Y129M-K244L、Y129M-K143Q-K244L、T38E-S258D、T38E-K143Q-S258D、P19E-Q184D、P19E-K143Q-Q184D、P19E-Q184L、P19E-K143Q-Q184L、N97D-G225C、N97D-K143Q-G225C、L60Q-Y61W、N97D-G225P、N97D-K143Q-G225P、N67D-P168S、N67D-K143Q-P168S、K63L-N71D、K63L-N71D-K143Q、K63R-N71D、T228V-Y235L、K143Q-T228V-Y235L、P19E-T38E-K63L-N71D-Y129M-Q184L-K244L-S258D-N261R;N67D-Y129M-P168S-Q184L-K244L-S258D-G259P;P19E-K63L-N67D-Q78D-K80T-N97D-Y129M-G225C-T228V-K244L;P19E-T38E-N67D-N97D-Y129M-P168S-Q184L-K244L-S258D-N261R;P19E-T38E-N67D-N71D-Q78D-K80T-N97D-Y129M-P168S-G225C-K244L-S258D-N261R;T38E-K63L-N71D-N97D-Y129M-Q184L-G225C-T228V-Q242L-K244L-S258D-N261R;P19E-K63L-N71D-N97D-Y129M-Q184L-G225C-K244L-S258D-G259P;N10T-T38E-S59V-L60Q-K63R-L66V-A68S-N74S-V75L-N97D-V103I-Y129M-F167Y-Q184L-A217P-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;P19E-T38E-N67D-N71D-N97D-Y129M-F167Y-Q184L-A217P-K244L-S258D-N261R;T38E-K63L-N67D-Q78D-K80T-N97D-Y129M-P168S-Q184L-K244L-S258D-N261R;P19E-T38E-N67D-Y129M-P168S-Q184L-K244L-S258D-N261R;P19E-N67D-N97D-Y129M-P168S-Q184L-K244L;P19E-T38E-K63L-N71D-Y129M-P168S-G225C-T228V-K244L-S258D-N261R;P19E-T38E-N67D-N97D-Q184L-A217P-G225C-T228V-Y235L-K244L-S258D-N261R;N10T-P19E-G28S-S30T-T38E-N67D-N71D-N97D-Y129M-P168S-Q184L-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;P19E-T38E-S59V-L60Q-K63R-N67D-N97D-V103I-Y129M-K143Q-F167Y-Q184L-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;P19E-T38E-N67D-N71D-Q78D-K80T-N97D-Y129M-P168S-G225C-T228V-K244L-S258D-N261R-Z298.01Q;P19E-T38E-S59V-L60Q-K63L-K70R-N71D-Q78D-K80T-N97D-E111D-Y129M-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-T38E-K63L-N71D-N97D-V103I-Y129M-F167Y-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-P19E-T38E-N67D-Q78D-K80T-N97D-Y129M-K143Q-Q184L-A217P-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-P19E-T38E-S59V-L60Q-K63L-N97D-V103I-Y129M-F167Y-Q184L-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;P19E-S30T-T38E-S59V-L60Q-K63R-N67D-N97D-V103I-Y129M-F167Y-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;P19E-S30T-T38E-S59V-L60Q-K63R-N67D-Q78D-K80T-N97D-I124V-Y129M-K143Q-F167Y-Q184L-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;N10S-P19E-S30T-T38E-S59V-L60Q-K63L-N67D-Q78H-K80T-I82M-N97D-Y129M-K143Q-F167Y-Q184L-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-P19E-S30T-T38E-S59V-L60Q-K63R-N67D-N97D-Y129M-K143Q-P168S-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;G4S-N10T-P19E-T38E-N67D-Q78D-K80T-N97D-Y129M-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-P19E-S30T-T38E-S59V-L60Q-K63L-K70R-N71D-Q78D-K80T-N97D-Y129M-T131A-F167Y-Q184L-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-P19E-S30T-T38E-S59V-L60Q-K63L-K70R-N71D-Q78D-K80T-N97D-E111D-Y129M-P168S-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;P19E-S30T-T38E-S59V-L60Q-K63R-N67D-N97D-Y129M-P168S-Q184L-K214I-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-P19E-S30T-T38E-S59V-L60Q-K63R-N67D-N97D-Y129M-K143Q-P168S-Q184L-G225P-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;M1V-P19E-S30T-T38E-T62E-N67D-N71D-Q78D-N97D-Y129M-K143R-F167Y-P168S-Q184L-G225C-Y235L-K244L-S258D-N261R-T284A-Z298.01Q;Y6E-N10T-P19E-G28S-S30T-T38E-K63L-N67D-N71D-N97D-E111S-Y129M-S135L-P168S-Q184L-G225C-T228V-Y235L-K244L-S258D-N261Q-D283S-Z298.01Q;N10T-P19E-S30T-T38E-S59V-L60Q-K63R-N67D-N71D-N97D-V103I-Y129M-K143Q-P168S-Q184L-G225P-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;A2S-P19E-G28S-S30T-T38E-K63R-N67D-N71D-N74E-K93R-N97D-Y129M-N150T-P168S-Q184L-N213A-G225C-Y235L-K244L-S258D-N261Q-Z298.01Q;M1L-N10T-P19E-G28A-S30T-T38E-K63L-N67D-N71D-Q78D-N97D-Y129M-A136L-P168A-Q184L-N213A-G225C-Y235L-K244L-S258D-N261R-Z298.01Q;P19E-T38E-S59V-K63R-N67D-N97D-V103I-Y129M-F167Y-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;N10T-P19E-G28A-S30T-T38E-K63R-N67D-N97D-Y129M-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Q;T3R-N10T-P19E-G28A-S30T-T38E-T62E-N67D-N71D-K93R-N97L-E111S-Y129M-D139M-P168S-Q184L-G225C-Y235L-K244L-S258D-N261Q-Z298.01Q;N10T-P19E-G28A-S30T-T38E-S59D-N67D-A68S-N71D-K93R-N97D-Y129M-K143Q-P168S-Q184D-G225C-Y235L-K244L-S258D-N261R-T284E-Z298.01Q;P19E-K63L-N71D-Y129M-P168S-Q184L-G225C-K244L-G259R;P19E-N67D-N71D-Q78D-K80T-N97D-Y129M-P168S-Q184L-K244L;P19E-T38E-N67D-Y129M-P168S-Q184L-T228V-K244L;P19E-T38E-N67D-Y129M-Q184L-K244L-S258D-N261R;P19E-K63L-N71D-Y129M-P168S-Q184L-K244L-S258D-N261R;P19E-T38E-K63L-N71D-Y129M-P168S-Q184L-K244L-S258D-G259P;K63L-N71D-Y129M-K143R-P168S-Q184L-G225C-T228V-K244L-S258D-G259P;又はP19E-T38E-K63L-N71D-Y129M-P168S-Q184L-K244L-S258D-N261Rを含み、
前記変異体、又はその組換えポリペプチド若しくは活性断片のアミノ酸位置は、配列番号14のアミノ酸配列との対応によって番号を付けられ、
前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片は、配列番号13のアミノ酸配列に対するアミノ酸配列同一性が少なくとも95%であり、
前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片は、前記基準ポリペプチドと比較して、1つ又は複数の特性が向上しており;特性の前記向上は、プロテアーゼの存在下での安定性の向上、洗剤又はバッファ中での安定性の向上、及び洗浄性能の向上から選択され、
特性の前記向上は、
(i)洗剤中またはバッファ中での安定性の向上であって、前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片は、約40℃~約70℃、約45℃~約65℃、約50℃~約60℃、約60℃~約70℃、又は約56℃の温度にて、少なくとも5分間、少なくとも10%、20%、30%、40%、又は50%の残留マンナナーゼ活性を保持する、向上;
(ii)プロテアーゼの存在下での安定性の向上であって、前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片は、プロテアーゼ及び/又は界面活性剤の存在下で、少なくとも15日間、又は約15~約40日間、マンナナーゼ活性を少なくとも50%保持する、向上;
(iii)洗浄性能の向上であって、前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片は、ローカストビーンガムの染みの洗浄PIが>1である、向上;並びに
(iv)所定時間経過後の洗浄性能の向上であって、前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片は、7時間後に洗浄活性が少なくとも15%残留しており、又は9時間後に洗浄活性が少なくとも11%残留している、向上
である、マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片。 - 前記改変は、P19E-S30T-T38E-S59V-L60Q-K63R-N67D-N97D-V103I-Y129M-F167Y-Q184L-G225C-T228V-Y235L-K244L-S258D-N261R-Z298.01Qであり;
前記変異体、又はその組換えポリペプチド若しくは活性断片のアミノ酸位置は、配列番号14のアミノ酸配列との対応によって番号を付けられている、請求項1に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片。 - 前記変異体、又はその組換えポリペプチド若しくは活性断片はさらに:
(i)位置31~40にてWXaKNDLXXAI(配列番号15)のモチーフ(式中、Xaは、F又はYであり、Xは、任意のアミノ酸である);
(ii)位置263~274にてLDXXXGPXGXLT(配列番号16)のモチーフ(式中、Xは、任意のアミノ酸である);
(iii)位置263~274にてLDX1V/AT/AGPX2GX3LT(配列番号17)のモチーフ(式中、X1は、M又はLであり、X2は、N、A、又はSであり、X3は、S、T、又はNである);及び
(iv)位置263~274にてLDM/LATGPN/AGS/TLT(配列番号18)のモチーフ
から選択される1つ又は複数のモチーフを含み、
前記変異体、又はその組換えポリペプチド若しくは活性断片のアミノ酸位置は、配列番号14のアミノ酸配列との対応によって番号を付けられている、請求項1または2に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片。 - 前記基準ポリペプチドは、GH5マンナナーゼであり、前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片は、GH5マンナナーゼ又はエンド-β-マンナナーゼである、請求項1~3のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片。
- 前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片はさらに、炭水化物-結合モジュールを含まない、請求項1~4のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片。
- 請求項1~5のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片を含む洗浄組成物。
- 少なくとも1つの界面活性剤;カルシウム及び亜鉛から選択される少なくとも1つのイオン;少なくとも1つの補助剤成分;少なくとも1つの安定化剤;約0.001重量%~約1.0重量%の、請求項1~5のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片;少なくとも1つの漂白剤;並びに/あるいはアシルトランスフェラーゼ、アミラーゼ、アルファ-アミラーゼ、ベータ-アミラーゼ、アルファ-ガラクトシダーゼ、アラビナーゼ、アラビノシダーゼ、アリールエステラーゼ、ベータ-ガラクトシダーゼ、ベータ-グルカナーゼ、カラギナーゼ、カタラーゼ、セロビオヒドラーゼ、セルラーゼ、コンドロイチナーゼ、クチナーゼ、エンド-ベータ-1,4-グルカナーゼ、エンド-ベータ-マンナナーゼ、エキソ-ベータ-マンナナーゼ、エステラーゼ、エキソ-マンナナーゼ、ガラクタナーゼ、グルコアミラーゼ、ヘミセルラーゼ、ヒアルロニダーゼ、ケラチナーゼ、ラッカーゼ、ラクターゼ、リグニナーゼ、リパーゼ、脂肪分解酵素、リポキシゲナーゼ、マンナナーゼ、オキシダーゼ、ペクチン酸リアーゼ、ペクチンアセチルエステラーゼ、ペクチナーゼ、ペントサナーゼ、ペルヒドロラーゼ、ペルオキシダーゼ、フェノールオキシダーゼ、ホスファターゼ、ホスホリパーゼ、フィターゼ、ポリガラクツロナーゼ、プロテアーゼ、プルラナーゼ、リダクターゼ、ラムノガラクツロナーゼ、ベータ-グルカナーゼ、タンナーゼ、トランスグルタミナーゼ、キシランアセチルエステラーゼ、キシラナーゼ、キシログルカナーゼ、キシロシダーゼ、メタロプロテアーゼ、及びそれら組合せから選択される少なくとも1つの酵素又は酵素誘導体:をさらに含む、請求項6に記載の洗浄組成物。
- 前記洗浄組成物は、(i)洗濯洗剤、布地柔軟仕上げ洗剤、食器洗い洗剤、及び硬質表面洗浄洗剤から選択される洗剤組成物、及び/又は、(ii)液体、粉末、顆粒状の固体、タブレット、シート、及び単位用量から選択される形態の組成物、及び/又は、(iii)ホスフェートを含有し、若しくはホスフェートを含有せず、且つ/又はホウ素を含有し、若しくはホウ素を含有しない、組成物である、請求項6又は7に記載の洗浄組成物。
- マンナンを含む汚れ又は染みを含む表面又はアイテムを、(i)請求項1~5のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片、あるいは(ii)請求項6~8のいずれか一項に記載の洗浄組成物と接触させることを含み、前記汚れ又は前記染みに含有される前記マンナンは加水分解される、洗浄方法
- 前記アイテムは、皿類又は布地である、請求項9に記載の洗浄方法。
- 請求項1~5のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片をコードする核酸配列を含むポリヌクレオチド。
- 請求項11に記載のポリヌクレオチドを含む発現ベクター。
- 請求項12に記載の発現ベクターを含む宿主細胞。
- 請求項1~5のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片を生産する方法であって:
(a)請求項12に記載の発現ベクターで請求項13に記載の宿主細胞を安定して形質転換することと、
(b)形質転換された前記宿主細胞を、前記宿主細胞が前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片を産生するのに適した条件下で培養することと;
(c)前記マンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片を回収することと、
を含む方法。 - 請求項1~5のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片を含む、食品組成物若しくは飼料組成物及び/又は食品添加物。
- 請求項1~5のいずれか一項に記載のマンナナーゼ変異体、又はその組換えポリペプチド若しくは活性断片の、食品組成物若しくは飼料組成物、並びに/又は食品添加物若しくは飼料添加物、並びに/又は食品若しくは飼料及び/若しくはペットフードの調製における使用。
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| US201662278387P | 2016-01-13 | 2016-01-13 | |
| US62/278,387 | 2016-01-13 | ||
| PCT/US2016/060844 WO2017079751A1 (en) | 2015-11-05 | 2016-11-07 | Paenibacillus sp. mannanases |
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-
2016
- 2016-11-07 JP JP2018522994A patent/JP7364331B2/ja active Active
- 2016-11-07 WO PCT/US2016/060844 patent/WO2017079751A1/en not_active Ceased
- 2016-11-07 CN CN201680070916.1A patent/CN109072208A/zh active Pending
- 2016-11-07 EP EP22165362.9A patent/EP4141113A1/en active Pending
- 2016-11-07 EP EP16801909.9A patent/EP3371308B1/en active Active
- 2016-11-07 US US15/773,290 patent/US20190153417A1/en not_active Abandoned
-
2020
- 2020-01-29 US US16/775,730 patent/US20200362324A1/en not_active Abandoned
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| Mannnase[Bacillus circulans],Genbank[online],2009.11.03,[retrieved on 2020.10.29],retrieved from the Internet,Accession AAX87003 |
Also Published As
| Publication number | Publication date |
|---|---|
| WO2017079751A1 (en) | 2017-05-11 |
| BR112018008946A2 (pt) | 2020-11-03 |
| EP3371308B1 (en) | 2022-05-11 |
| EP3371308A1 (en) | 2018-09-12 |
| JP2019501636A (ja) | 2019-01-24 |
| CN109072208A (zh) | 2018-12-21 |
| US20200362324A1 (en) | 2020-11-19 |
| EP4141113A1 (en) | 2023-03-01 |
| US20190153417A1 (en) | 2019-05-23 |
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