JPH0348699A - 二特異性およびオリゴ特異性の一価およびオリゴ価リセプター、それらの調整および使用 - Google Patents
二特異性およびオリゴ特異性の一価およびオリゴ価リセプター、それらの調整および使用Info
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- JPH0348699A JPH0348699A JP2165485A JP16548590A JPH0348699A JP H0348699 A JPH0348699 A JP H0348699A JP 2165485 A JP2165485 A JP 2165485A JP 16548590 A JP16548590 A JP 16548590A JP H0348699 A JPH0348699 A JP H0348699A
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Abstract
め要約のデータは記録されません。
Description
上の異なる特異性の抗体のF (ab)断片をコードす
るDNAの融合による遺伝子操作によって調製される、
二特異性(bispecific)およびオリゴ特異性
(oli8ospecific)の−価(monova
l ent)およびオリゴ価(of igovale
nt)リセブターに間する。これに関して、一つの特異
性は、好ましくは、細胞膜上または間隙に位置している
種度関連抗原(TAA)のエピトープに向けられるかま
たは腫瘍内皮(TE)のエピトープに向けられるが、そ
の他の特異性は高分子量または低分子量のリガンド(I
igand)に関連して、例えば、キレートのエチレ
ンジアミン四酢酸塩(ethylenediamine
tetra−acetate)およびジエチレントリア
ミン五酢酸塩(diethylenetriamine
penta−acetate)のY90複合型(各々、
EDTA−Y2OおよびDTPA−Y2O)と反応する
。特に好ましい態様においては、キレートとの結合は、
fos−jun相互作用(または他にはアビデイン−ビ
オチン(avidin−biotin)相互作用)を介
して、キレートリセブターの腕部(arm)上で起きる
。他の好ましい特異性は、触媒的な性質を有する、ある
いは同じ腫瘍細胞上の他のTAAとまたはリンパ球細胞
上のリセプターと結合する。
。
)リンカ−を介する多種(diverse)特異性の抗
体の化学的結合 ()1. Paulus: Behr
ingnst、Mitt、78.118−132.19
.85)既に人手可能で、種々のモノクローナル抗体(
MA b )を分泌するバイブリドの融合、および二特
異性の一価の部分の単離(U、S。
、 Nat1、 Acad、 Sci、 USA 83
.1453−1457.1986)二つの異なるMAb
の重鎖および軽鎖遺伝子(4個の遺伝子)のネズミミエ
ローマ細胞または他の真核細胞発現系へのトランスフェ
クション、および二特異性−価部分の単離(u、 Zi
mmermann: Rev、 Physio、 Bi
ochem。
8G、 J、 vanDijkら:lnt、 J、 C
ancer 43.344−349.1989)この型
の二特異性抗体は、悪性腫瘍の治療および診断に用いら
れる。方法の原理は、第一′段階において、長期にわた
って大量投与量で二特異性巨大分子(macromol
ecule)を注射することによって、標的細胞上で二
つの特異性の中の一つによって認識されるエピトープの
飽和を達成することからなる。
的に吸着した二特異性抗体の非標的Mi織からの自己除
去(autoel 1m1nation)がある。この
自己除去は、糖残基、好ましくはガラクト−ス、に結合
している抗イデイオタイプ抗体の注射によって加速する
ことができ、二特異性リセプターの抗l!瘍腕部に対し
て向けられる。
子量リガンドの静脈内注射からなるが、このリガンドは
、細胞内で蓄積せず、体内停留時間が短く、911Y、
ll16Re、IflllRe、+89Re199I
ITcまたは口I 1 nなどのβ−“およびγ−エミ
ッターの複合定数(complexing const
ant)が高く、かつ二特異性すセブタ一の第二の特異
性に高い親和性で結合する。この段階の結果、標的組織
上での保持が延長されるとともに放射性リガンドの濃縮
が行われ、その結果、標的組織の選択的崩壊がなされて
、例えば、転移(metastases)の診断が可能
になる。
たはオリゴ価結合部位を有しており、過当なリンカ−に
よる遺伝子操作によって産生される、二特異性およびオ
リゴ特異性リセブターを今提供する。
ードする遺伝子断片を、例中の表1に示されるような過
当な合成オリゴヌクレオチドを用いて、MAbbのV8
ドメイン(domain)のN末端をポリペプチドスペ
ーサーを介してMAbaのCH1ドメインのC末端に共
有結合で結合させるようにして、連結させる(第1図)
。v14aCH1a−ポリペプチドスペーサー−VHb
CHl b遺伝子構築物を、抗体aおよびbの軽鎖の遺
伝子とともに真核細胞(例えばマウスミエローマ細胞)
にトランスフェクト(transfect)させるo
C)Il a、 C,1b、 C,aおよびC,bドメ
インを、反対荷電が定常ドメイン(C+1 a (+
) Cxa ()、CHlb(−)CKb (+))(
+、:陽性、−=陰性)と接触領域で合わさるように、
または、接触の反対領域が各場合に疎水性または各場合
に親水性であるようにして、修飾する。これは、トラン
スフェクトされたもの(形質転換体、transfec
tomas)が、重鎮および軽鎖の正しい対合を有する
バイブリド分子を選択的に発現することを意味する(第
2図)。
低分子量りガント、好ましくはキレートDTPA−Y9
0またはEDTA−Y2O、に対する抗体を表すもので
ある。
当なリンカ−を介しての、多種特異性の抗体のv8およ
びCHlドメインの遺伝子工学的な構築を意味し、これ
によれば、対応する軽鎖との結合のための要求される移
動性(mobility)が存在して、抗原結合が妨げ
られない。
たは結合部位と呼ばれる。二特異性−価リセプターは、
したがって、二つの特異性がある場合には各場合に一つ
の抗原結合部位を有する。したがって、二特異性三価リ
セプターは、一つの特異性のための一つの抗原結合部位
を、他の特異性のために二つの抗原結合部位を各々有す
る。
Y2O(MAb b)に対して一価である二特異性リ
セプターを、上記のオリゴヌクレオチドリンカーを用い
て、上記の重鎮遺伝子構築物をMAbaの■8およびC
,1ドメインをコードする遺伝子部分に連結させること
によって調製して(第3図)、ポリペプチドスペーサー
によ7てMAb bのCHlドメインのC末端をMA
baのvHドメインのN−末端に連結するようにする。
鎖の遺伝子とともに真核細胞(例えばミエローマ細胞)
にトランスフェクトさせる。上記のようにして、C,4
1およびC,ドメインは、相補的な荷電または各場合に
疎水性または親水性である接触領域とともに提供される
。形質転換体は、MAbaの二つのF (ab)断片お
よびMAb bの一つのF (ab)断片(第4図)
を含む融合分子を選択的に発現する。ペプチドリンカ−
の移動性は、MAbaの二つのF (ab)腕部の腫瘍
細胞に対する整列(aiignment)、同時に、細
胞間空間に対するMAb bのF (ab)腕部の整
列を可能にする。同様に、同一または異なる特異性のさ
らなる結合部位を加えることが可能である。さらに、構
築物中の特異性の配列(5equence)を自由に組
み合わせることが可能である。
な、細胞膜上または間隙中に位置するエピトープのため
の特異性と、細胞外空間にのみ分布する低分子量または
高分子量リガンドのための特異性とを共に有する、二特
異性またはオリゴ特異性、−価またはオリゴリセブター
に間する。これに関連して、一つの特異性は、独国特許
出願第93909799.4号明細書において提示され
たように、好ましくは腫瘍特異性抗体によって形成され
、他の特異性は、好ましくは、DTPA−Y2Oまたは
E D T A−Y 90に対して向けられる。特に好
ましい態様においては、結合はキレートと、fos−j
un相互作用(例5を参照されたい)を介してキレート
リセブター腕部上で起きる。他の好ましい本発明の変形
は、触媒的活性を有する特異性の組み入れからなる。さ
らに、二つの特異性を有する三価の第4図の例で示され
るように、特異性の配列または結合価の選択に制限はな
い。
または5の■遺伝子を含むものである。
許出願第p 3909799.4号明細書に記載されて
いる。さらに、相補性決定領域(CDR)は、Kaba
tおよびWu (Sequences of Prot
eins ofImmunological Inte
rest、 US Dept、 of )Iealth
and Human 5ervices、 US Go
vernment PrintingOffice、1
987)の方法によって同定することができる。同様に
好ましい構築物は、上記のモノクローナル抗体によフて
定義されたエピトープに対する特異性を含むものである
。
工学的方法、および標的細胞の抑制および診断のための
医薬物の調製のための上記構築物の使用に間する。すな
わち、第一の段階において、構築物を注射した後に標的
細胞上で関連エピトープを飽和させて、次いで、非特異
的に吸着したあるいは非結合の構築物を除去する。これ
に続く次の段階は、注射および次いでの低または高分子
量リガンドの特異的結合からなるが、このリガンドは、
細胞内に蓄積されず、本質的に細胞毒性(cytoto
xic)または適宜に他の段階において身体外(ext
racorporeal)の影響によッテ細胞毒性に「
活性化」されるものである。この型の方法の例は、酵業
的活性化、プロドラッグのマイクロ波照射による活性化
またはレーザー光線による活性化などがある。
通りである。
MAbの調製 イソチオシアネートベンジル−DTPA(化学式2式% 法によってヒト血清アルブミン(HSA、キャリアとし
て)に、H9A分子当り19個のベンジル−DTPAの
誘導化(derivatization)率で、ハブテ
ンとして共有結合させた。冷却したYを中に複合させて
おいたこのハブテン−キャリア複合体の20μgを、0
日目にフロイントのアジュバントとともに、7日および
14日目に不完全フロインドアジュバントとともに、お
よび21日目にPBSとともに、Ba1b/cマウスに
皮下注射した。
マウスの牌臓を、SP210−Ag14ミエローマ細胞
系(Shulmanら: Nature 276.26
9.1978)と融合させた。得られるバイプリドーマ
を、DTPAおよびEDTAに対する高親和性のMAb
の産生についてDTPA−特異性ELISA中で試験し
た。ELISAは、HSA−ベンジル−DTPA−Yを
含む溶液を負荷した固相からなる。
の金属イオン複合体と予備インキュベートしてから、特
異的固相との結合を測定した。抗−マウス免疫グロブリ
ン抗体と結合している酵素増幅系を、この目的のために
用いた。これらの方法の詳細は付録1aおよび1bに記
載の通りである。
用いて得られた。
、これらMAbは、APAAP技法((ordel l
ら: J、 )Iistochem、 Cytoch
em、 32.219.1984)を用いて見出された
ように、冷温保存された( cryopreserve
d)組織上で正常ヒト組織と結合しない。したがって、
これらのMAbをインビボで診断および治療に用いるこ
とが可能である。
、キレ−)DTPAおよびEDTAの非−複合および複
合型(付録1c)である。
および1.2−ジアミノエタンをインヒビタ、−として
用いたく付録1eを参照されたい)。
ており、池のMAb全てと対照的に、EDTA−Yへの
選択的結合を示す(付録1e。
と他のEDTA複合体のより高い過剰量、を参照された
い〉。バイブリド2050/174を、したがって、安
定化させて、二特異性リセプターにおけるEDTA−Y
腕部を作出するのに用いた。
1遺伝子構築物の調製および発現 ここで用いた技法は、特に記載がない限り、Mo1ec
ular Cloning、A Laboratory
Manua1、Sambrook、 Fr1tsc
h、 Maniatis、 Co1d 5pri
n8tlarbor Laboratory、 198
2 (pp、 11−44.51−127.133−1
34.141S146.150−167.170.18
8−193、+97−199.248−255.270
−294.310−328.364−401.437−
506)およびMo1ecular Cloning、
ALaboratory Manua1、5econ
d Edition、 Sambrook。
pring HarborLaboratory Pr
ess、 1989 (pp、16.2−16.22.
16.30−16.40.16.54−16.55)か
ら採用した。
M、 Fr1schauf ら : J、 M
o1. Bio1、 170 、827−842.
1983およびG、H,A、 Seemannら: T
he EMBOJournal 5.547−552.
1986)中のヒト遺伝子バンクから単離した。
(第5図)、他方でCH1エクソンおよびHLAB27
遺伝子の3°NT領域を含む(第6図、プラスミドM中
の断片M)、構築物をこのIgG、C遺伝子から独国特
許出願第P 3825615.0号明細書に記載のよう
にして調製した。
よびbのm RN Aから0rlandiら(Proc
。
833−3837.1989)による記載のようにして
増幅させて、M13ベクター中でクローニングした(V
Ha PCRおよびVHb PCR)(第7図)。
て真核細胞発現ベクターp E V)l (Simon
ら二Nuc1、Ac1ds Res。
図)。
c遺伝子サブクローン(第5図)は、CH1エクソンと
ヒンジエクソンとの間にPstl切断部位を含む。■8
遺伝子は、5′末端にPstl切断部位を含む。リンカ
−オリゴヌクレオチドは、それが5′末端でIgGC遺
伝子のCH1+IHサブフラグメント上のPstI切断
部位領域および3゛末端でv、b遺伝子のPstl切断
部位と、重複(overlap)するように設計されて
いる。リンカ−オリゴヌクレオチドは、そのPstI切
断部位によってPUC18プラスミドのPstl切断部
位にクローニングされる(第9図)。結果としてプラス
ミドクローンLが得られる。
3C遺伝子サブフラグメントを有するプラスミドを、P
stIおよびBamHIで切断して、V、4bPCRか
らPs t I−BamHI断片として切り出したVH
b遺伝子断片に連結させる(第10図)。その結果、プ
ラスミドXが得られる。
同様にPstlで切り出しておいたリンカ−断片に連結
させる(第11図)。核酸配列分析を用いて、リンカ−
が、正しい位置方向でC8lとvHbとの間にイントロ
ン3とリンカ−エクソン間のイントロン/エクソン結合
部を損なわず、かつ、リンカ−とV。b遺伝子間の結合
部における解読枠を損なわずにクローニングされている
、クローンZを同定する。
スミドMからBamHIで切り出しておいた断片Mと連
結させる。制限酵素分析を用いて、断片Mを正しい位置
方向で含んでいるクローンYを同定する(第12図)。
末端を埋填した後に、プラスミドXからHindIII
およびBamHI切断によって切り出した断片(C□1
−リンカー−v、b)に連結する。ヌクレオチド配列分
析および制限地図作出を用いて、全てのエクソンを正し
い位置方向で有する融合遺伝子VHa C,1−リンカ
ー−vHb c、iを含むブラスミドクローンPEV
Tを同定する(第13図)。
(ab)融合タンパク質を発現させるために、抗体a
およびbの軽鎖の遺伝子を有するプラスミドとともに過
当な真核発現細胞にトランスフェクトさせる。
4遺伝子)のトランスフェクション免疫グロブリン遺伝
子の単離は、独国特許出願第P 3909799.4号
明細書に記載されている。
状にした後にエレクトロポレーション(electro
poration)によってX63Ag8.653ミエ
ローマ細胞(tL 5topperら:Biochem
、 Biophys、 Acta 900.38−44
.1987)中にトランスフェクトさせた。選択培地中
で増殖した形質転換体を、特異的RIA中で二特異性−
価MAbの産生について試験した。このRIAは、カゼ
インによる非特異的部位のブロックの後、分析される形
質転換体上清を上に位置させた同相上に吸着させたTA
Aからなった。9[lYまたは991ITcと複合して
いるDTPAまたはEDTAを加えてから過剰分を洗い
流した後、二特異性−価抗−TAAX抗−EDTA M
Abを分泌したこれら形質転換体を、固相上の増加した
放射性シグナルによって検出することが可能であった。
させて細胞培養中に広げた。細胞培養上清を、IOXに
濃縮して、MAb画分をタンパク質Aクロマトグラフィ
ー(P、L、 i:、yら:mmunochemist
ry 15.429.1978)によって精製し、二特
異性−価MAbを含む両分をアニオン交換クロマトグラ
フィー (J、 Van Dijkら: Int、 J
。
って精製した。
50/174)を含む精製タンパク質を、500μ8の
投与量で0.3.5.8.10および12日ICヒトl
[異種移植片(xenograf ts)(CoCa4
)を有するヌードマウスに静脈内注射した。27〜30
日目の各動物にEDTA−Y2Oの5071Ciを静脈
内注射した。第二のグループの動物には同じ日に二特異
性MAbの代わりに500 It gのMAb BW
431/26、およびEDTA−Y90注射を上記のよ
うに行った。
A−Y2Oの代わりにPBS(腫瘍増殖コントロールと
して)を注射した。腫瘍の増殖を6週間追跡した。ED
TA−Y2Oの注射の結果、二特異性−価MAbを注射
されたグループにおいて1[の増殖の有意の阻害が認め
られたが、一方、MAb BW431/26を注射し
て、EDTA−Y2Oで処理した動物では、PBSのみ
を注射された動物と同じく、腫瘍増殖の阻害がみられな
かった・ これらのデータは、毒性素因(principle)と
してEDTA−Y2Oと組合せて二特異性−価MAbの
選択的腫瘍治療効果を示す。
性またはオリゴ特異性リセプターによって得られる。な
ぜならば、これらはTAAとの二価結合のために腫瘍上
により長く保持され、したがって、リガンドが同様に腫
瘍上により長く、より高濃度で保持されるからである。
)を増加させることによる、二特異性またはオリゴ特異
性巨大分子の生物学的有効性の最適化細胞外分布をして
いる親水性キレートのオリゴ特異性巨大分子の抗−キレ
ート腕部への効果的な付着に影響する決定的な因子は、
キレートへのこの腕部の強い要求性である。モノクロー
ナル抗体のそれらの対応するエピトープへの強い要求性
は、105〜10111/molの範囲である。これら
の結合強度は、効果的なラジオイムノセラピー(rad
ioimmunotherapy)に必要な量のキレー
トを腫瘍上に位置させるにはあるいは不十分であること
から、次の例においては、fos−ロイシン−ジッパ−
(z i pper)ペプチド(fos−ペプチド)と
jun−ロイシン−ジッパ−ペプチド(jun−ペプチ
ド) (Erinに、 O’5heraら: 5ci
ence、 245、1989)とのきわめて強い相互
作用を用いて、キレートをできるだけ強固に抗−キレー
ト腕部上に固定化した。この強力なfos−jun相互
作用を利用することができるように、好ましくは、fo
s−ペプチドを共有結合でキレート(DTPA)に連結
させることが必要である。この目的のために、第一の手
段においてイソチオシアネートベンジル−DTPAをヒ
ドラジン(またはジアミノアルカン)と反応させること
が可能である。このようにして産生されたDTPA−ベ
ンジルチオカルバジドを、第二段階において、N−(γ
−マレイミドブチリルオキシ)サクシニミドまたは類似
体と反応させて、DTPA−ベンジル−(γ−マレイミ
ドブチリル)チオカルバジドを得ることができる。次い
で、第三の段階で、この化合物をグリシン−グリシン−
システィン(第1図)によって広げておいたfos−ペ
プチドに、アミノ末端のシスティンの遊離のSH基を介
して連結させる。このようにして産生されたfos−ペ
プチド−DTPA抱合体(conjugate)を、第
四段階において、塩化イツトリウム(yttrium)
と複合化させる。このようにして産生されたfos−ペ
プチド−DTPA−Y抱合複合体を、次いでニーまたは
オリゴ特異性巨大分子のjun−ペプチド腕部へのイン
ビボ添加に用いることができる。以上略述した例の合成
を以下に詳述する。
n−EDTA) (30mg、 54μmol)を10
%(V/V)水成ヒドラジン中で1時間攪拌した。次い
で、溶媒を高真空下で除去して、残留物を五酸化リン上
で高真空下で乾燥させて、最後に凍結乾燥した。産生物
をDO讐EX讐X 2 (H”型)で中和して、再び凍
結乾燥した(収!28mg)。
(20mg、34μmol)およびN−(r−マレイミ
ドブチリルオキシ)サクシニミド(8m8.29μmo
l=0.9等量)を無水ジメチルフォルムアミド中で1
時間攪拌した。混合物を、次いで、蒸発させて乾燥して
、残留物を高真空下で乾燥した。
段階3.1を参照されたい)の燐酸緩衝生理食塩水(2
ml)を、段階2で得られた産生物混合物(4mg)の
ジメチルフォルムアミド(400μm)懸濁液と混合し
て、室温で1時間インキュベートした。反応混合物を、
次いで、燐酸緩衝生理食塩水中でセファデックス015
カラム上でのゲル濾過に供した。
収f14.2mg)。
のアミノ酸配列 各アルファベット文字は次のアミノ酸を表す。
E=グルタミン酸、G=ニブリシン■=イソロイシン、
K=リジン、L=ロイシン、M=メチオニン、N=アス
パラギン、Q=グルタミン、R=アルギニン、S=セリ
ン、T=スレオニン、■=バリン、Y=チロシン。
d Biosystems Model 430A)を
用いてタート−ブチルオキシカルボニル保護基を用いる
Merrifield固相法(StewartおよびY
oun8:5olid Phase 5ynthesi
s%Pierce Chemical(ompany、
第二板Rockford ’I11.)によって合成し
た。オリゴペプチドを、フェニルアセタミドメチル−ポ
リスチレン支持体から切り出した。保護基(Tomら:
J、 Am、 Chem、 Soc、 105.64
42−6455、+983)を除去した後、オリゴペプ
チドをRivierら(J、 Chromatogra
phy 288.303−328.1984)による記
載の逆相クロマトグラフィー(PepRPCカラム、P
harmacia社製)によって精製した。
TA抱合体(4,2mg)を、等張生理食塩水10.1
Mクエン酸ナトリウム(pH7,0)に対して、分子f
l1、000の排除限界(exclusionlimi
t)を有する透析チューブ(スペクトラム)中で透析し
て、3mlの等張生理食塩水10.1Mクエン酸ナトリ
ウム(pH7,0)に溶解した6mgの塩化イツトリウ
ムと混合した。1時間後、燐酸緩衝生理食塩水に対して
逆透析を行って、キレート溶液を一30℃で保存した。
ツトリウムキレートを次いt、°高い要求性で二特異性
またはオリゴ:特異性巨大分子のjun−ペプチド腕部
と結合させるために、リガンドとして用いる。特にこの
相互作用に適している二特異性巨大分子の構築は、次の
例に記載されている。
tisら (Laboratory Manual
EMBL、 1982、He1delber:g)お
よびSambrook (MolecularClon
ing: A Laboratory Manual)
から採用した。
、 Fr1schaufら: J、 Mo1. Bio
1、 170.827−842.1983およびG、H
,A、 Seemannら: The EMBOJou
rnal 5.547−552.1986)中のヒト遺
伝子バンクから単離した。1gG3C遺伝子のCHIエ
クソンおよび最初のヒンジエクソンのみを含む構築物(
D)(第14図)を、この1gG3C遺伝子から独国特
許出願第P 3B25615.0号明細書に記載のよう
にして調製した。
同じく独国特許出願第P 3825615.0号明細書
に記載のようにして調製した。C3エクソンおよびHL
A B27に遺伝子の3’ NT領領域みを含む構築物
(E)(第15図)を、このHLA B27に遺伝子か
ら調製した。
Vi域をプラスミドEからXbalで切り出して、断片
を単離して、構築物りのXbaI切断部位にクローニン
グした。制限酵素分析および核酸配列分析を用いて、C
3エクソンおよびHLA B27に遺伝子の3’ NT
領領域正しい5’−3’の位置方向で含む、3′がIg
G3C遺伝子断片からである、クローンFを同定した(
第16図)。
mおよびEcoRIを用いてプラスミドから切り出して
、M13mp18二本鎖(DS)ファージのHindm
とEcoRI切断部位切断部位−ニングする。抗体/H
LA融合遺伝子断片を含むファージクローンGを単離す
る(第17図)。
d、 5cience、 U、S、A。
c)オリゴヌクレオチド1および2(表6)とハイブリ
ダイズさせて、オリゴヌクレオチド間の間隙をフレノウ
DNAポリメラーゼおよびT4リガーゼで閉環させた。
酵素分析および核酸配列分析を用いて、ヒンジエクソン
の5′末端における5stl制限酵素切断部位が除去さ
れたファージクローン(G)を同定した。同時に、5s
tIおよび5phI制限酵素切断部位を、ヒンジエクソ
ンの3′末端に導入したく第18図)。5stI切断部
位を除去するためにヒンジエクソンの第二のコドンの3
番目の塩基をCからGに変換して、5stIおよび5p
hI切断部位を導入するために塩基群5 ’ GAGC
TCGGGGCA3 ’をヒンジエクソンの15番目と
16番目のコドンの間に導入したく表7)。
完全に5stlで部分的に切断する。
8)を合わせて、その各末端に5phlおよび5stI
制限酵素切断部位の切断部を含み、Junロイシンジッ
パ−(0’5heaら: 5cience。
コードする、二本鎖DNA断片が得られる。
よびsph I制限酵素切断部位にクローニングして、
ヒンジエクソン中にJ u nジッパ−ペプチドのため
の配列が挿入された遺伝子構造物を含むファージクロー
ンHな同定する(第19図)。
indlIIおよびEcoRIで切り出して、末端をT
4ポリメラーゼで埋填して、SmaI−切断KsFベク
ター(Strata3ene、 11099 Nort
hTorrey Pines Road%La Jol
la Ca1ifornia 92037)中にクロー
ニングした。抗体/Jun/HLA融合遺伝子をその両
側をBamHI切断部位で挟むように位置して含む、プ
ラスミドクローンlを同定した(第20図)。
からBamHIで切り出して、特異的機能性免疫グロブ
リン■遺伝子を含む発現プラスミドp A B S t
o p (Behringwerke AG)中にク
ローニングした。特異的■遺伝子を、特許出願第P、3
909799.4号明細書に記載のようにして得る。抗
体/Jun/HLA!合遺伝子構築物を正しい位置方向
でvH遺伝子の下流に含む発現プラスミドKを、同定し
た(第21図)。
むプラスミドおよび耐性(resistance)遺伝
子を有するプラスミドの共形質転換(cotransf
ormation)によって、ヒンジ領域に二つのJu
nジッパ−ペプチドを含み、もはやいかなるホモダイマ
ー(homodimer) (J u n / J
u n)形成のないようにJunジッパ−ペプチドが修
飾されている、特異的抗体F (ab’) 2断片の発
現が導かれる。
a)による固体腫瘍の浸透(penetration)
は援慢に起き、通常、縁辺領域または腫瘍の少ない領域
のみに達することを示している。これらの研究調査は、
少量の巨大分子の一回の注射からなる実験に基づいてい
る。これに対して、本発明者らは、ヌードマウス異種移
植片における全腫瘍体の実質的な侵透が多量の二特異性
またはオリゴ特異性リセブターの反復的な静脈内注射(
10X250μgリセブター/マウス、10日間)によ
って可能であることを見、出した。さらに、これら′の
TAAへの特異的結合の故に二特異性またはオリゴ特異
性リセブターは、腫瘍細胞膜上および腫瘍間隙中で長期
の開く〉20日)大量に付着したままで保持される。こ
れらの結果は、ヒト直腸および膵臓腫瘍異種移植片の冷
温保存された( cryopreserved)薄切片
に間接的アルカリフォスファターゼ技法を用いて得られ
た。
性リセブター分子は、崩壊および排除によってTAA−
陰性正常組織および血液から既に除去されていた。この
除去期間を短縮するために非結合の二特異性またはオリ
ゴ特異性リセブター分子の抗−TAA腕部とのみ反応す
る抗−イディオタイプMAb(抗Id)をニーまたはオ
リゴ特異性リセブターの10回の注射の完了後24時間
に静脈内注射した。この−回の注射は、非結合ニーまた
はオリゴ特異性リセブター分子の血液からの除去を速め
て、肝臓および牌臓における代謝率を高めた。
をニーまたはオリゴ特異性リセブターの浸透および結合
相の完了後わずか4日後に注射することが可能である。
導かれたものである。
オリゴ特異性リセブターの静脈内注射b) 11日n1
1×50μgの抗1dの静脈内注射 c) 14日l1治療的投与量のEDTA−Y2Oの
静脈内注射 ヌードマウスと腫瘍患者における比較的免疫シンチグラ
フ(immunoscintigraphic)データ
に基づいて、この方法は、ヒトにおいても腫瘍治療に適
していると考えられる。しかし、ヒト系において注射さ
れるべき量は、範囲が異なる(10X5〜10gの二特
異性すセブタ−lX1gの抗Id)。抗1dの注射は、
治療には必ずしも必須ではない。
イタープレート(U型)タイプB、 Nunc社製、N
o、4−60445 1) 1.+1g抱合体/mlP B S (p H
7,2)の濃度の50μlのY−ベンジル−DTPA−
H9A19抱合体を、各ウェルにピペットで入れて、室
温で一晩インキユベートする。
)リスクエン酸塩緩衝液(pH7,4)(洗浄溶液1)
で洗浄する(1回洗浄=250μm/ウェルの洗浄液を
ウェルに入れて2分間静置してから吸引によ)て除去す
る)。
合には、それをセルロース上に室温で一装置く(開口部
を下にして)。次いでプレートを、乾燥カートリッジ(
Gaplast社製、Po5trach 529.81
00 Garmisch−Partenkirchen
)とともにフィルムに密閉する。プレートを、+4℃で
これらの条件下で少なくとも8週間保存することができ
る。
ェルに入れて、37℃で30分間インキュベートする。
との予備インキュベーションをブロッキングの開に行う
(付録2を参照されたい)。
トした試験すべきハイブリドーマ上清を、各ウェルζこ
入れて、室温で30分間インキニーベートする。
らブロッキング溶液て1:500に希釈しておいたヤギ
抗−マウスI gG、抗体50 /lIを各ウェルに入
れて、室温で30分間インキュベートする。
3回洗浄を行う。
る。
行う。
幅系を次のようにして作る。
)を混合して、1部のジアホラーゼ(d 1aphor
ase)と1部のADHをピペットで入れる。
ウェル当り100μmのOol NH2SO4溶液によ
って反応を停止させる。
92 runで吸光度(extinction)を測定
する。50μmのNADPと50μmの溶液および12
00μmの0.1 NH2SO4をブランクとして用い
る。
攪拌してカゼイン3%濃度にして、pHを7.4に調整
する。次いで4.OOOrpmで10分間遠心分離して
粒子を除去する。
ァターゼ(Southern Biotechnolo
gyAssociates社製、カタログ番号1080
−04)で標識する。
ス、0 、1 mM M g S Oa (pH9,5
)に溶解する。
LIUM Violet)の調製:2 、5 mg/m
lの30%エタノールを超音波槽で溶解する。常に新鮮
なものを調製する。
を少量づつに分けて一20℃で保存する。
づつに分けて一20℃で保存する。
の定量ELISA系を用いて決定することができる。
をCa”およびMg″″′″を含まないPBS中で1.
25713/mlに希釈する。
10−6g −xモル1.25μg =x
=8.33X40−12モルMAbとインヒビターの1
+1比を得るために、8.33X 10−12モル/2
00μm(これは5の係数(factor)で増える)
の濃度のインヒビターの10 )i lを、8.33X
10−’2モル/mlの濃度のハイブリドーマ上清の
50 /Z lに加える。
0倍、50,000倍、10,000倍、5.000倍
、1,000倍および100倍の濃度で室温で30分間
インキュベートする。この50μ+を、ピペットでEL
ISA、(付録1aのno。
000倍過剰となる。より低いコンペティターとMAb
比は、コンペティター溶液を特別な塩イオン溶液で所望
のモル過剰に適宜に希釈することによって達成された(
付録1bを参照されたい)。
複合定数は著しく高いために、これら金属イオンとのD
TPAまたはEDTAの等モル混合では完全な飽和が期
待されねばならない。このために、対応する金属イオン
を、DTPAまたはEDTAと3倍モル過剰量でインキ
ュベートした。
二度蒸留水溶液)(付録1dを参照されたい)を30μ
mの1028モルDTPA保存溶液(二度蒸留水溶液)
と室温で5分間インキュベートした。このコンペティタ
ー溶液10 /11をバイブリドーマ上清と混合するこ
とによって、コンベティタ硫酸カドミウム Riedel de )Iaen 塩化亜鉛 メルク社製 次の金属イオンの10ミリモル溶液を、二度蒸留水中に
調製した。
の過剰モル MAb No+ 2050/174 20501531 20501532 20501534 20501535 MAb No。
10” 10” 5xlO’ 103102 5xlO’ 10310” 5xlO’ 10” 10” 10’ 10” 10” DTPA−Cd DTPA−Zn 10” 5xlO3 10” 5x103 10” 5xlO3 10” 5xlO3 10” 103 DTPA−Cu xlO3 5xlO’ xlO3 xlO3 03 DTPA−Pb 1、スー シ′7ミノ トラン
ス−19ン 7コ;7トゐ1DTA−Y EDTA−にn 7Jし 了Jし xlO3 5xlO” 5xlO” 03 EDTA−Cu 03 02 xlO3 03 02 EDTA−Pb X103 10’ 10’ xlO3 02 DTPA 州曝
スペーサーによる結合構造を示す説明図ろる。 12図および第4図は、それぞれ第1図および3図のも
のに軽鎖が対合した構造を示す説明図)る。 第5図〜第13図はVllaCHl−リンカ−V)ll
bcH1遺伝子構築物の構築を示す説明図である。 第14図〜第21図はMab−jun融合分子のための
プラスミドにの構築を示す説明図である。
Claims (1)
- 【特許請求の範囲】 1、二つまたはそれ以上の異なる特異性の抗体のV_H
およびC_H1領域をコードするDNAの過当なリンカ
ーによる融合およびそれらに属する軽鎖のための遺伝子
部分と合わせての発現系における続いての発現による遺
伝子操作によって、得ることができる、二特異性または
オリゴ特異性の一価またはオリゴ価リセプター 2、一つの特異性が動物またはヒト腫瘍関連抗原に対し
て向けられている、請求項1に記載のリセプター。 3、一つの特異性が触媒的または酵素的活性を有する、
請求項1に記載のリセプター。 4、一つの特異性が動物またはヒト腫瘍関連抗原に対し
て向けられており、他の一つの特異性がキレートに向け
られている、請求項1に記載のリセプター。 5、キレート結合がfos−jun相互作用を介してリ
セプターキレート腕部で起きる、請求項4に記載のリセ
プター。 6、一つの特異性が表2、3、4または5に示される可
変領域を有するモノクローナル抗体に由来する、請求項
1、2、4または5に記載のリセプター。 7、三つの結合部位が二つの特異性の場合に存在する、
請求項1、2、4、5または6に記載のリセプター。 8、四つの結合部位が二つの特異性の場合に存在する、
請求項1、2、4、5または6に記載のリセプター。 9、三つの特異性の場合、一つが腫瘍に向けられて、他
の二つが異なるやり方でDTPAまたはEDTAに向け
られている、請求項1、2、4、5または6に記載のリ
セプター。10、重鎖抗体部分をコードするDNA断片
を リンカーを用いて連結して、軽鎖のための遺伝子
とともに発現系で発現することからなる、請求項 1、
2、3、4、5または6に記載のリセプター の製造法
。 11、医薬物としての、請求項1〜9のいずれ か1項
に記載のリセプター。
Applications Claiming Priority (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| DE3920358.1 | 1989-06-22 | ||
| DE3920358A DE3920358A1 (de) | 1989-06-22 | 1989-06-22 | Bispezifische und oligospezifische, mono- und oligovalente antikoerperkonstrukte, ihre herstellung und verwendung |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| JPH0348699A true JPH0348699A (ja) | 1991-03-01 |
| JP2978210B2 JP2978210B2 (ja) | 1999-11-15 |
Family
ID=6383263
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| JP2165485A Expired - Lifetime JP2978210B2 (ja) | 1989-06-22 | 1990-06-22 | 二特異性およびオリゴ特異性の一価およびオリゴ価リセプター、それらの調整および使用 |
Country Status (14)
| Country | Link |
|---|---|
| US (1) | US5591828A (ja) |
| EP (1) | EP0404097B1 (ja) |
| JP (1) | JP2978210B2 (ja) |
| KR (1) | KR0183980B1 (ja) |
| AT (1) | ATE142230T1 (ja) |
| AU (1) | AU639241B2 (ja) |
| CA (1) | CA2019559C (ja) |
| DE (2) | DE3920358A1 (ja) |
| DK (1) | DK0404097T3 (ja) |
| ES (1) | ES2093623T3 (ja) |
| GR (1) | GR3021109T3 (ja) |
| IE (1) | IE76715B1 (ja) |
| PT (1) | PT94443B (ja) |
| RU (1) | RU2096459C1 (ja) |
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1990
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- 1990-06-20 DK DK90111640.0T patent/DK0404097T3/da active
- 1990-06-20 DE DE59010480T patent/DE59010480D1/de not_active Expired - Lifetime
- 1990-06-20 EP EP90111640A patent/EP0404097B1/de not_active Expired - Lifetime
- 1990-06-20 ES ES90111640T patent/ES2093623T3/es not_active Expired - Lifetime
- 1990-06-21 PT PT94443A patent/PT94443B/pt not_active IP Right Cessation
- 1990-06-21 IE IE225490A patent/IE76715B1/en not_active IP Right Cessation
- 1990-06-21 RU SU904831122A patent/RU2096459C1/ru active
- 1990-06-21 CA CA002019559A patent/CA2019559C/en not_active Expired - Lifetime
- 1990-06-21 AU AU57621/90A patent/AU639241B2/en not_active Expired
- 1990-06-22 KR KR1019900009252A patent/KR0183980B1/ko not_active Expired - Lifetime
- 1990-06-22 JP JP2165485A patent/JP2978210B2/ja not_active Expired - Lifetime
-
1994
- 1994-09-29 US US08/317,612 patent/US5591828A/en not_active Expired - Lifetime
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1996
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Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| JPH05219960A (ja) * | 1991-03-27 | 1993-08-31 | F Hoffmann La Roche Ag | キメラポリペプチド |
| JP2006509744A (ja) * | 2002-11-14 | 2006-03-23 | ブラッコ イメージング エッセ ピ ア | 変化したタンパク質を細胞表面に呈示する腫瘍の診断および処置のための薬剤 |
Also Published As
| Publication number | Publication date |
|---|---|
| DE59010480D1 (de) | 1996-10-10 |
| CA2019559C (en) | 2002-01-08 |
| JP2978210B2 (ja) | 1999-11-15 |
| CA2019559A1 (en) | 1990-12-22 |
| EP0404097B1 (de) | 1996-09-04 |
| ATE142230T1 (de) | 1996-09-15 |
| US5591828A (en) | 1997-01-07 |
| DK0404097T3 (ja) | 1997-02-10 |
| ES2093623T3 (es) | 1997-01-01 |
| IE76715B1 (en) | 1997-10-22 |
| IE902254L (en) | 1990-12-22 |
| DE3920358A1 (de) | 1991-01-17 |
| KR910001057A (ko) | 1991-01-30 |
| AU5762190A (en) | 1991-01-03 |
| PT94443A (pt) | 1991-02-08 |
| KR0183980B1 (ko) | 1999-04-01 |
| EP0404097A2 (de) | 1990-12-27 |
| AU639241B2 (en) | 1993-07-22 |
| IE902254A1 (en) | 1991-01-16 |
| GR3021109T3 (en) | 1996-12-31 |
| PT94443B (pt) | 1997-02-28 |
| EP0404097A3 (de) | 1991-10-23 |
| RU2096459C1 (ru) | 1997-11-20 |
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