JP2010215657A - N末端化学修飾タンパク質組成物および方法 - Google Patents
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Abstract
【解決手段】ホウ水素化ナトリウム、シアノホウ水素化ナトリウムなどの還元剤を使用する還元的アルキル反応を用いて、タンパク質のN末端のα−アミノ酸をデキストラン、ポリ(N−ビニルピロリドン)、ポリエチレングリコール類のような水溶性ポリマーで選択的に修飾し、モノポリマー/タンパク質結合体の実質的に均質で、安定なタンパク質を含む組成物の製造方法を提供する。
【選択図】なし
Description
組換えヒトmet−G−CSF(本明細書では“rhG−CSF”または“r−met−hu−G−CSF”と呼ぶ)は、上述のようにSouza特許、米国特許第4,810,643号にある方法に従って調製した。この特許は参考として本明細書に組み入れる。使用したrhG−CSFは、以下に示す(DNA配列によってコードされる)アミノ酸配列をもつE.coli由来の組換え発現産物であった(配列番号1および2):
10mg/mlの上記rh−G−CSF溶液を100mM Bicine pH8.0に溶かした溶液を、平均分子量が6000ダルトンの固体のSCM−MPEG(カルボキシメチルメトキシポリエチレングリコールのN−ヒドロキシスクシニミジルエステル)(Union Carbide)に添加した。これによってrh−G−CSFよりもSCM−MPEGが1.5モル過剰になった。1時間軽く攪拌した後、滅菌水で混合液を2mg/mlに希釈し、希釈したHClによってpHを4.0に調整した。反応は室温で起こさせた。この段階で反応混合物は主に3形態のモノPEG化rh−G−CSFから構成されており、その他、ジPEG化rh−G−CSF、未修飾のrh−G−CSF、および反応の副産物(N−ヒドロキシスクシニミド)が含まれていた。
3形態のモノPEG化rh−G−CSFは、イオン交換クロマトグラフィによって別々に分離した。反応混合液を、緩衝液A(20mM酢酸ナトリウム、pH4.0)で平衡化しているPharmacia SセファロースFFカラム(Pharmacia XK50/30リザーバ、ベッド容量440ml)に添加した(1mg蛋白質/ml樹脂)。カラムを3カラム容量の緩衝液Aで洗浄した。蛋白質は0〜23%の直線勾配の緩衝液B(20mM酢酸ナトリウム、pH4.0、1M NaCl)を15カラム容量用いて溶出した。次に1カラム容量の100%緩衝液Bでカラムを洗浄し、3カラム容量の緩衝液Aで再度平衡化させた。操作全体の流速は8ml/分に維持した。溶離剤を280nmでモニターし、5mlの分画を収集した。モノPEG化した個々の分子種を含む分画は、図1Aに従ってプールした。このようにプールした液をYM10 76mmメンブランを使った350mL Amicon攪拌セルを使って濃縮した。
各サンプルの特性を知るために5種類の分析を実施した:(1)SDS−Page(図1B)、(2)サイズ排除クロマトグラフィHPLC(“SEC HPLC”)(図2)、(3)ペプチドマッピング分析(図3A、3B、3C)、(4)in vitro G−CSFバイオアッセイ(図4)、および(5)ハムスターを用いたin vivo試験(図5Aおよび5B)。
**この分子種は使用したアッセイ条件下では不安定であることに注意。
1.SDS−PAGE。SDS−PAGEは非還元4〜20% ISSDaiichi Pure Chemicals(東京)のミニゲルにおいて、コーマシーブリリアントブルーR−250染色剤を用いて実施された。ゲルはImage Quantを用いた動的分子濃度計によってスキャンした。結果:結果は図1Bに示してある。レーン番号1(左から数えて)には蛋白質の分子量標準(Novex Mark 12分子量標準)が入っていた。レーン2には3μgのrh−G− CSF標準が含まれている。レーン3には10μgのSCM−PEG−GCSF反応混合液が入っている。レーン4には10μgのN末端モノPEG化G−CSFが含まれている。レーン5にはN末端のメチオニンからの35番目の残基に見出されたリジンにPEG化したモノPEG化G−CSFが10μg入っている。レーン6にはN末端のメチオニンから41番目の残基に見出されたリジンにPEG化したモノPEG化G−CSFが10μg含まれている。図から分かるように、N末端にモノ PEG化した物質が含まれているレーン3はバンドが一つである。
結果:図2から分かるように、N末端にモノPEG化したrh−G−CSFを含むライン“C”はピークが1個であり、ライン“D”(リジン35にモノPEG化した物質)および“E”(リジン41にモノPEG化した物質)もやはりピークが1個であった。これはモノPEG化G−CSFから分離した分画は純度が実質的に高いことを示している。
E.安定性試験
更に、上述のように調製したN末端およびリジン35にモノPEG化した分子種について、安定性試験を実施した。(リジン41物質は、活性が未修飾G−CSFを上回らないことが実証されたため使用しなかった)。これらの試験によって、N末端にPEG化したG−CSFがもう一方のモノPEG化G−CSFであるモノPEG化リジン35と比べて、保管中に予想外に安定していることが実証された。安定性はSEC−HPLCを使って視覚化させた生成物の分解という点で評価した。
20mMのNaCNBH3 を含む100mMのリン酸ナトリウム(pH5)中の、冷却し(4℃)攪拌したrhG−CSF溶液(1ml、5mg/ml、上記実施例のところで説明済み)に、5倍モル過剰のメトキシポリエチレングリコールアルデヒド(MPEG)(平均分子量、6kDa)を加えた。同じ温度で反応混合物を攪拌し続けた。
1.分子量
モノPEG化結合体における分子量は、SDS−PAGE、ゲル濾過、マトリックスアシステッドレーザーデソープション質量分析、平衡遠心分離によって求めた。結果は以下の表4に示した。
PEG化MPEG−GCSF結合体のin vitro生物学的活性は、3Hチミジンのマウス骨髄細胞への刺激取り込みを測定することによって求めた。
2種類の化学的方法(アミドvs還元アルキル化のアミン)によって調製したN末端にPEG化したG−CSFの凝集程度を比較した。予想外のことだが、アミン化学を用いてN末端にPEG化したG−CSFは、アミド結合によってN末端にPEG化したG−CSFよりもかなり安定していることが分かった(NHS化学反応は実施例1に説明済み)。
モノPEG化コンセンサスインターフェロンの調製には、米国特許第4,695,623号(この全体を参照として本明細書に組み入れる)の図2にあるIFN−αcon1(本明細書ではIFN−con1と呼ぶ)を使用した。IFN−con1は細菌内での外因性DNAの発現によって生成されたもので、N末端にメチオニル残基を持っていた。
20mMのNaCNBH3を含む、冷却し(4℃)攪拌しておいた100mMのリン酸ナトリウム中のIFN−con1溶液、pH4.0(3.45mg/ml、N末端がブロックされた形態を32.25%含む)に、8倍モル過剰のメトキシポリエチレングリコールアルデヒド(MPEG)(平均分子量12kDa)を加えた。
1.均質性
精製したモノ−MPEG−IFN−Con1結合体の均質性は、10〜20%または4〜20%プレキャストグラジェントゲル(Integrated Separation Systems)を用いたSDS−PAGEによって調べた。分子量35kDaのところにメインバンドが現れた。
モノ−MPEG−IFN−Con1結合体のin vitro生物学的活性は、その抗ウイルス生物活性を測定することによって決定した。モノ−MPEG−IFN−Con1結合体のin vitro生物学的活性は、ヒト(HeLa)細胞におけるその抗ウイルス生物活性を測定することによって決定した。
予め除去したN末端ブロック分子の一部を持つ上述のIFN−con1に対しても、本還元アルキル化を実施した。上述のように還元アルキル化法にはPEG 12000とPEG 20000の両方を用いた。
モノMPEG−IFN−con1:総面積の66%(265.93mlで溶出)
蛋白質凝集物およびオリゴMPEG−IFN−con1結合体:総面積の24%(238.42mlで溶出)
未反応のIFN−con1:総面積の10%(328.77mlで溶出)。
Claims (5)
- 単一の反応性アルデヒド基を有する水溶性ポリマーをタンパク質に結合させる方法であって、
(a)還元アルキル化反応の条件下、該タンパク質部分のリジン残基のε−アミノ基がプロトン化される一方でN−末端のα−アミノ基がプロトン化されないpH条件下で、タンパク質を水溶性ポリマーと反応させて、前記水溶性ポリマーを前記N−末端α−アミノ基に選択的に結合させ、
(b)反応生成物を得、次いで
(c)任意に、反応生成物を未反応部分から分離する、ことを含んでなる方法。 - 前記ポリマーが医薬的に許容できる請求項1記載の方法。
- 前記水溶性ポリマーが、デキストラン、ポリ(n−ビニルピロリドン)、ポリエチレングリコール類、プロピレングリコールホモポリマー類、ポリプロピレンオキシド/エチレンオキシドコポリマー類、ポリオキシエチル化ポリオール類およびポリビニルアルコール類からなる群から選択される請求項1記載の方法。
- 前記ポリマーがポリエチレングリコールである請求項3記載の方法。
- 前記還元アルキル化反応に、ホウ水素化ナトリウム、シアノホウ水素化ナトリウム、ホウ酸ジメチルアミン、ホウ酸トリメチルアミンおよびホウ酸ピリジンから選択される還元剤を使用する請求項1記載の方法。
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US08/321,510 US5824784A (en) | 1994-10-12 | 1994-10-12 | N-terminally chemically modified protein compositions and methods |
US321,510 | 1994-10-12 |
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JP2005286188A Division JP2006077021A (ja) | 1994-10-12 | 2005-09-30 | N末端化学修飾タンパク質組成物および方法 |
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JP2010215657A true JP2010215657A (ja) | 2010-09-30 |
JP2010215657A5 JP2010215657A5 (ja) | 2011-08-25 |
JP5350330B2 JP5350330B2 (ja) | 2013-11-27 |
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JP51319196A Expired - Lifetime JP3177251B2 (ja) | 1994-10-12 | 1995-02-08 | N末端化学修飾タンパク質組成物および方法 |
JP19257696A Expired - Lifetime JP3177449B2 (ja) | 1994-10-12 | 1996-07-22 | 水溶性ポリマーで修飾したコンセンサスインターフェロン |
JP11076959A Pending JPH11310600A (ja) | 1994-10-12 | 1999-03-19 | N末端化学修飾タンパク質組成物および方法 |
JP2002288746A Withdrawn JP2003155299A (ja) | 1994-10-12 | 2002-10-01 | N末端化学修飾タンパク質組成物および方法 |
JP2003106520A Pending JP2003327600A (ja) | 1994-10-12 | 2003-04-10 | N末端化学修飾タンパク質組成物および方法 |
JP2005286189A Withdrawn JP2006045243A (ja) | 1994-10-12 | 2005-09-30 | N末端化学修飾タンパク質組成物および方法 |
JP2005286188A Withdrawn JP2006077021A (ja) | 1994-10-12 | 2005-09-30 | N末端化学修飾タンパク質組成物および方法 |
JP2010134726A Expired - Lifetime JP5350330B2 (ja) | 1994-10-12 | 2010-06-14 | N末端化学修飾タンパク質組成物および方法 |
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JP19257696A Expired - Lifetime JP3177449B2 (ja) | 1994-10-12 | 1996-07-22 | 水溶性ポリマーで修飾したコンセンサスインターフェロン |
JP11076959A Pending JPH11310600A (ja) | 1994-10-12 | 1999-03-19 | N末端化学修飾タンパク質組成物および方法 |
JP2002288746A Withdrawn JP2003155299A (ja) | 1994-10-12 | 2002-10-01 | N末端化学修飾タンパク質組成物および方法 |
JP2003106520A Pending JP2003327600A (ja) | 1994-10-12 | 2003-04-10 | N末端化学修飾タンパク質組成物および方法 |
JP2005286189A Withdrawn JP2006045243A (ja) | 1994-10-12 | 2005-09-30 | N末端化学修飾タンパク質組成物および方法 |
JP2005286188A Withdrawn JP2006077021A (ja) | 1994-10-12 | 2005-09-30 | N末端化学修飾タンパク質組成物および方法 |
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US (7) | US5824784A (ja) |
EP (5) | EP0822199B1 (ja) |
JP (8) | JP3177251B2 (ja) |
KR (2) | KR100248111B1 (ja) |
CN (4) | CN1896103A (ja) |
AT (2) | ATE179991T1 (ja) |
CA (3) | CA2178752C (ja) |
DE (3) | DE10299044I1 (ja) |
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