JP2018500271A - 細菌株を含む組成物 - Google Patents
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Abstract
Description
本発明の組成物は、エンテロコッカス・ガリナラム種の細菌株を含む。実施例は、この種の細菌が、がんを治療又は予防するために有用であることを実証している。
(i)L−アラビノース、D−リボース、D−キシロース、D−ガラクトース、D−グルコース、D−フルクトース、D−マンノース、N−アセチルグルコサミン、アミグダリン、アルブチン、サリシン、D−セロビオース、D−マルトース、スクロース、D−トレハロース、ゲンチオビオース、D−タガトース及びグルコン酸カリウムの少なくとも1つ(例えば、少なくとも2、3、4、5、6、7、8、9、10、11、12、13、14、15、16、17又は全て)の発酵に対して陽性、並びに/又は
(ii)D−マンニトール、メチル−αD−グルコピラノシド(Methyl-αD-glycopyranoside)、D−ラクトース、デンプン及びL−フコースの少なくとも1つ(例えば、少なくとも2、3、4又は全て)の発酵に対して中間
であり、好ましくは、それらの決定は、API50CHL分析(好ましくは、bioMerieux社のAPI50CHLパネルを使用)による。
(i)マンノース発酵、グルタミン酸デカルボキシラーゼ、アルギニンアリールアミダーゼ、フェニルアラニンアリールアミダーゼ、ピログルタミン酸アリールアミダーゼ、チロシンアリールアミダーゼ、ヒスチジンアリールアミダーゼ及びセリンアリールアミダーゼの少なくとも1つ(例えば、少なくとも2、3、4、5、6、7又は全て)に対して陽性、並びに/又は
(ii)β−ガラクトシダーゼ−6−ホスフェート、β−グルコシダーゼ及びN−アセチル−β−グルコサミニダーゼの少なくとも1つ(例えば、少なくとも2又は全て)に対して中間、並びに/又は
(iii)ラフィノース発酵、プロリンアリールアミダーゼ、ロイシルグリシンアリールアミダーゼ、ロイシンアリールアミダーゼ、アラニンアリールアミダーゼ、グリシンアリールアミダーゼ及びグルタミルグルタミン酸アリールアミダーゼの少なくとも1つ(例えば、少なくとも2、3、4、5、6又は全て)に対して陰性
であり、好ましくは、それらの決定は、炭水化物、アミノ酸及び硝酸塩の代謝アッセイにより、並びにアルカリホスファターゼ活性分析によるものでもよく、より好ましくはRapid ID 32A分析(好ましくは、bioMerieux社のRapid ID 32A系を使用)による。
(i)グリシンアリールアミダーゼ、ラフィノース発酵、プロリンアリールアミダーゼ、及びロイシンアリールアミダーゼの少なくとも1つ(例えば、少なくとも2、3又は4つ全て)に対して陰性であり、例えば、それらの決定は、炭水化物、アミノ酸及び硝酸塩の代謝アッセイにより、好ましくはRapid ID 32A分析(好ましくは、bioMerieux社のRapid ID 32A系を使用)により;並びに/又は
(ii)L−フコースの発酵に対して中間陽性であり、好ましくは、それらの決定は、API50CHL分析(好ましくは、bioMerieux社のAPI50CHLパネルを使用)による。
好ましい実施形態において、本発明の組成物は、がんの治療又は予防に使用するための組成物である。実施例は、本発明の組成物の投与が、いくつかの腫瘍モデルで腫瘍増殖の低減を導くことができることを実証している。
IMMU-132(Immunomedics社製);E7449(Eisai社製);Thermodox(Celsion社製);Cometriq(Exellxis社製);Lonsurf(Taiho Pharmaceuticals社製);Camptosar(Pfizer社製);UFT(Taiho Pharmaceuticals社製);及びTS-1(Taiho Pharmaceuticals社製)。
好ましくは、本発明の組成物は、本発明の細菌株を腸管へ送達及び/又は部分的若しくは全体的に定着させるために胃腸管に投与される。一般に、本発明の組成物は経口により投与されるが、直腸的に、鼻内に、又は頬側若しくは舌下経路を介して投与されてもよい。
一般に、本発明の組成物は、細菌を含む。本発明の好ましい実施形態において、組成物は、フリーズドライ形態で製剤化されている。例えば、本発明の組成物は、本発明の細菌株を含む顆粒又はゼラチンカプセル、例えばハードゼラチンカプセルを含みうる。
本発明に使用するための細菌株は、標準的な微生物学技術、例えば、参照文献Handbook of Microbiological Media, Fourth Edition (2010) Ronald Atlas, CRC Press、Maintaining Cultures for Biotechnology and Industry (1996) Jennie C. Hunter-Cevera, Academic Press、Strobel (2009) Methods Mol Biol. 581:247-61に詳細に記載の技術を使用して培養することができる。
本発明者らは、本発明の細菌株が、がんを治療及び予防するために有用であることを明らかにした。これは、本発明の細菌株が宿主免疫系に与える効果の結果と考えられる。したがって、本発明の組成物は、ワクチン組成物として投与されるとき、がんを予防するためにも有用でありうる。特定のそのような実施形態において、本発明の細菌株は生存している。特定のそのような実施形態において、本発明の細菌株は、腸管に部分的又は全体的に定着することができる。特定のそのような実施形態において、本発明の細菌株は生存しており、腸管に部分的又は全体的に定着することができる。他の特定のそのような実施形態において、本発明の細菌株は、殺傷、不活化又は減弱化されていてもよい。特定のそのような実施形態において、組成物は、ワクチンアジュバントを含んでもよい。特定の実施形態において、組成物は、注射、例えば、皮下注射を介した投与のためのものである。
本発明の実施は、別段の記載がない限り、化学、生化学、分子生物学、免疫学及び薬理学の従来の方法を当該分野の技能の範囲内で利用しうる。そのような技術は、文献において十分に説明されている。例えば、参照文献Gennaro (2000) Remington: The Science and Practice of Pharmacy. 20th edition, ISBN: 0683306472及びMolecular Biology Techniques: An Intensive Laboratory Course, (Ream et al., eds., 1998, Academic Press)、Methods In Enzymology (S. Colowick and N. Kaplan, eds., Academic Press, Inc.)、Handbook of Experimental Immunology, Vols. I IV (D.M. Weir and C.C. Blackwell, eds, 1986, Blackwell Scientific Publications)、Sambrook et al. (2001) Molecular Cloning: A Laboratory Manual, 3rd edition (Cold Spring Harbor Laboratory Press)、Handbook of Surface and Colloidal Chemistry (Birdi, K.S. ed., CRC Press, 1997)、Ausubel et al. (eds) (2002) Short protocols in molecular biology, 5th edition (Current Protocols)、PCR (Introduction to Biotechniques Series), 2nd ed. (Newton & Graham eds., 1997, Springer Verlag)などを参照。
概要
この試験では、本発明による細菌株を含む組成物の有効性を、4種の腫瘍モデルで試験した。
被検物質 − 細菌株#MRX518
リファレンス物質 − 抗CTLA−4抗体(クローン:9H10、カタログ:BE0131、アイソタイプ:シリアンハムスターIgG1、Bioxcell社製)。
・10mLのYCFAを(調製した10mLのE&O lab社製ボトルから)Hungateチューブにピペッティングする
・チューブを密封し、シリンジインプットを使用してCO2でフラッシュし、系を使い切る
・Hungateチューブをオートクレーブする
・冷却されるとき、Hungateチューブに、1mLのグリセロール原液を接種する
・チューブを、静止した37℃インキュベータ内に約16時間置く
・翌日、この継代培養物を1mL取り、10mLのYCFA(事前に加温され、再度フラッシュされたHungateチューブ、全て2連)に接種する
・それらを、静止した37℃インキュベータ内に5〜6時間置く。
使用した細胞株の詳細を下記表に示す:
抗腫瘍活性、EMT6モデル
処置スケジュール − 最初の投与開始を0日目とした。0日目に、Vivo manager(登録商標)ソフトウェア(Biosystemes社製、クテルノン、仏国)を使用して、個々の体重に応じて非移植マウスをランダムに9/8匹の群にした。0日目に、マウスは、媒体(培養培地)又は細菌株を受けた。14日目に、全てのマウスに、下記のようにEMT−6腫瘍細胞を移植した。24日目に、陽性対照群のマウスは、抗CTLA−4抗体処置を受けた。
処置スケジュール−最初の投与開始を0日目とした。0日目に、Vivo manager(登録商標)ソフトウェア(Biosystemes社製、クテルノン、仏国)を使用して、個々の体重に応じて非移植マウスをランダムに9/8匹の7つの群にした。0日目に、マウスは、媒体(培養培地)又は細菌株を受ける。14日目に、全てのマウスに、下記のようにLL/2腫瘍細胞を移植した。27日目に、陽性対照群のマウスは、抗CTLA−4抗体処置を受けた。
処置スケジュール−最初の投与開始を0日目とした。0日目に、Vivo manager(登録商標)ソフトウェア(Biosystemes社製、クテルノン、仏国)を使用して、個々の体重に応じて非移植マウスをランダムに9匹の7つの群にした。0日目に、マウスは、媒体(培養培地)又は細菌株を受けた。14日目に、全てのマウスに、下記のようにHepa1−6腫瘍細胞を移植した。16日目に、陽性対照群のマウスは、抗CTLA−4抗体処置を受けた。
臨床的モニタリング − 腫瘍の長さ及び幅を、週に2回カリパスで測定し、腫瘍の容量を次式により見積もった(Simpson-Herren and Lloyd (1970) Cancer Chemother Rep. 54:143-74):
抗腫瘍活性、EMT6モデル
結果を図1に示す。本発明の細菌株を用いた処置は、両方の陰性対照と比較して、腫瘍容量の明らかな低減を導いた。陽性対照では、予想されたように、腫瘍容量の低減も導かれた。
結果を図2に示す。本発明の細菌株を用いた処置は、両方の陰性対照と比較して、腫瘍容量の明らかな低減を導いた。
結果を図3に示す。未処置陰性対照群は、この群が他の群よりも肝重量が少なかったために、予想されたような態様ではない。しかしながら、媒体陰性対照群及び陽性対照群は、媒体のみで処置したマウスが抗CTLA4抗体で処置したマウスよりも肝臓が大きく、媒体陰性対照群で腫瘍負荷がより大きいことを反映していたために、いずれも予想された態様を示した。本発明の細菌株を用いた治療は、媒体陰性対照群のマウスと比較して肝重量(したがって腫瘍負荷)の明らかな低減を導いた。
細菌MRX518の純粋な培養物をPCR遺伝子分析で試験した。実験には2つのアームがあった:1)MRX518を、ヒト結腸細胞(CaCo2)と共培養して、宿主に対する細菌の効果を調査した、及び2)MRX518を、IL1で刺激したCaCo2細胞と共培養し、炎症環境における細菌の効果を模倣した。両方のシナリオにおける効果は、遺伝子発現分析を通じて評価した。結果を以下に示す。
本明細書に記載の少なくとも1つの細菌株を含む本明細書に記載の組成物を、密封容器中に25℃又は4℃で保存し、容器を30%、40%、50%、60%、70%、75%、80%、90%又は95%の相対湿度を有する雰囲気中に置く。1カ月、2カ月、3カ月、6カ月、1年、1.5年、2年、2.5年又は3年後、標準的プロトコルで決定されるコロニー形成単位で測定される細菌株が、少なくとも50%、60%、70%、80%又は90%残存する。
概要
この試験では、MRX518細菌株単独及びリポ多糖(LPS)との組合せでの、未熟樹状細胞におけるサイトカイン産生に対する効果を試験した。
これらの試験の結果は、図4a〜dで見ることができる。MRX518単独の添加は、陰性対照と比較して、サイトカインIL−6及びTNF−αのレベルの実質的な増加を導く(図4a及びc)。LPS(陽性対照)の添加は、陰性対照と比較して、IL−6及びTNF−αのレベルの増加を導くが、IL−1βについては増加を導かない(図4b)。MRX518とLPSとの組合せは、産生されるIL−1βのレベルの相乗的増加を導いた(図4d)。
MRX518は、未熟樹状細胞におけるIL−6及びTNF−αサイトカイン産生をより高く誘導する能力を有する。LPSとMRX518との組合せは、未熟樹状細胞においてサイトカインIL−1βのレベルを増加させることができる。これらのデータは、MRX518が単独又はLPSとの組合せで、炎症促進によりがんを抑制可能な炎症性サイトカインIL−1β、IL−6及びTNF−αを増加させることができることを示している。MRX518の単独又は組合せでの処置は、腫瘍増殖を制限することのできるサイトカインを誘導することができる。
概要
この試験では、MRX518細菌株単独及びLPSとの組合せでの、単球及びマクロファージについてのモデル細胞株であるTHP−1細胞のサイトカイン産生に対する効果を試験した。
これらの試験の結果は、図5a〜cで見ることができる。LPSなしでのMRX518の添加は、細菌なし及び細菌沈降対照と比較して、IL−1β、IL−6及びTNF−αのサイトカインレベルの増加を導く。LPS及びMRX518の添加は、サイトカイン産生の相乗的増加を導く。
MRX518は、THP−1細胞におけるサイトカイン産生を誘導させる能力を有し、この産生は、LPSの添加により、相乗的に増加させることができる。これらのデータは、MRX518が単独又はLPSとの組合せで、炎症促進によりがんを抑制可能な炎症性サイトカインIL−1β、IL−6及びTNF−αを増加させることができることを示している。MRX518の単独又は組合せでの処置は、腫瘍増殖を制限することのできるサイトカインを誘導することができる。
配列番号1(エンテロコッカス・ガリナラム16S rRNA遺伝子−AF039900)
1 taatacatgc aagtcgaacg ctttttcttt caccggagct tgctccaccg aaagaaaaag
61 agtggcgaac gggtgagtaa cacgtgggta acctgcccat cagaagggga taacacttgg
121 aaacaggtgc taataccgta taacactatt ttccgcatgg aagaaagttg aaaggcgctt
181 ttgcgtcact gatggatgga cccgcggtgc attagctagt tggtgaggta acggctcacc
241 aaggccacga tgcatagccg acctgagagg gtgatcggcc acactgggac tgagacacgg
301 cccagactcc tacgggaggc agcagtaggg aatcttcggc aatggacgaa agtctgaccg
361 agcaacgccg cgtgagtgaa gaaggttttc ggatcgtaaa actctgttgt tagagaagaa
421 caaggatgag agtagaacgt tcatcccttg acggtatcta accagaaagc cacggctaac
481 tacgtgccag cagccgcggt aatacgtagg tggcaagcgt tgtccggatt tattgggcgt
541 aaagcgagcg caggcggttt cttaagtctg atgtgaaagc ccccggctca accggggagg
601 gtcattggaa actgggagac ttgagtgcag aagaggagag tggaattcca tgtgtagcgg
661 tgaaatgcgt agatatatgg aggaacacca gtggcgaagg cggctctctg gtctgtaact
721 gacgctgagg ctcgaaagcg tggggagcga acaggattag ataccctggt agtccacgcc
781 gtaaacgatg agtgctaagt gttggagggt ttccgccctt cagtgctgca gcaaacgcat
841 taagcactcc gcctggggag tacgaccgca aggttgaaac tcaaaggaat tgacgggggc
901 ccgcacaagc ggtggagcat gtggtttaat tcgaagcaac gcgaagaacc ttaccaggtc
961 ttgacatcct ttgaccactc tagagataga gcttcccctt cgggggcaaa gtgacaggtg
1021 gtgcatggtt gtcgtcagct cgtgtcgtga gatgttgggt taagtcccgc aacgagcgca
1081 acccttattg ttagttgcca tcatttagtt gggcactcta gcgagactgc cggtgacaaa
1141 ccggaggaag gtggggatga cgtcaaatca tcatgcccct tatgacctgg gctacacacg
1201 tgctacaatg ggaagtacaa cgagttgcga agtcgcgagg ctaagctaat ctcttaaagc
1261 ttctctcagt tcggattgta ggctgcaact cgcctacatg aagccggaat cgctagtaat
1321 cgcggatcag cacgccgcgg tgaatacgtt cccgggcctt gtacacaccg cccgtcacac
1381 cacgagagtt tgtaacaccc gaagtcggtg aggtaacctt tttggagcca gccgcctaag
1441 gtgggataga tgattggggt gaagtcgtaa caaggtagcc gtatcggaag gtgcggctgg
1501 atcacc
配列番号2(エンテロコッカス・ガリナラムMRX518株の16S rRNAのコンセンサス配列)
TGCTATACATGCAGTCGAACGCTTTTTCTTTCACCGGAGCTTGCTCCACCGAAAGAAAAAGAGTGGCGAACGGGTGAGTAACACGTGGGTAACCTGCCCATCAGAAGGGGATAACACTTGGAAACAGGTGCTAATACCGTATAACACTATTTTCCGCATGGAAGAAAGTTGAAAGGCGCTTTTGCGTCACTGATGGATGGACCCGCGGTGCATTAGCTAGTTGGTGAGGTAACGGCTCACCAAGGCCACGATGCATAGCCGACCTGAGAGGGTGATCGGCCACACTGGGACTGAGACACGGCCCAGACTCCTACGGGAGGCAGCAGTAGGGAATCTTCGGCAATGGACGAAAGTCTGACCGAGCAACGCCGCGTGAGTGAAGAAGGTTTTCGGATCGTAAAACTCTGTTGTTAGAGAAGAACAAGGATGAGAGTAGAACGTTCATCCCTTGACGGTATCTAACCAGAAAGCCACGGCTAACTACGTGCCAGCAGCCGCGGTAATACGTAGGTGGCAAGCGTTGTCCGGATTTATTGGGCGTAAAGCGAGCGCAGGCGGTTTCTTAAGTCTGATGTGAAAGCCCCCGGCTCAACCGGGGAGGGTCATTGGAAACTGGGAGACTTGAGTGCAGAAGAGGAGAGTGGAATTCCATGTGTAGCGGTGAAATGCGTAGATATATGGAGGAACACCAGTGGCGAAGGCGGCTCTCTGGTCTGTAACTGACGCTGAGGCTCGAAAGCGTGGGGAGCGAACAGGATTAGATACCCTGGTAGTCCACGCCGTAAACGATGAGTGCTAAGTGTTGGAGGGTTTCCGCCCTTCAGTGCTGCAGCAAACGCATTAAGCACTCCGCCTGGGGAGTACGACCGCAAGGTTGAAACTCAAAGGAATTGACGGGGGCCCGCACAAGCGGTGGAGCATGTGGTTTAATTCGAAGCAACGCGAAGAACCTTACCAGGTCTTGACATCCTTTGACCACTCTAGAGATAGAGCTTCCCCTTCGGGGGCAAAGTGACAGGTGGTGCATGGTTGTCGTCAGCTCGTGTCGTGAGATGTTGGGTTAAGTCCCGCAACGAGCGCAACCCTTATTGTTAGTTGCCATCATTTAGTTGGGCACTCTAGCGAGACTGCCGGTGACAAACCGGAGGAAGGTGGGGATGACGTCAAATCATCATGCCCCTTATGACCTGGGCTACACACGTGCTACAATGGGAAGTACAACGAGTTGCGAAGTCGCGAGGCTAAGCTAATCTCTTAAAGCTTCTCTCAGTTCGGATTGTAGGCTGCAACTCGCCTACATGAAGCCGGAATCGCTAGTAATCGCGGATCAGCACGCCGCGGTGAATACGTTCCCGGGCCTTGTACACACCGCCCGTCACACCACGAGAGTTTGTAACACCCGAAGTCGGTGAGGTAACCTTTTTGGAGCCAGCCGCCTAAGGTG
配列番号3(MRX518株の染色体の配列)−電子形式配列表参照。
配列番号4(MRX518株のプラスミドの配列)−電子形式配列表参照。
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Claims (25)
- がんを治療又は予防する方法に使用するための、配列番号2と少なくとも95%同一である16s rRNA配列を有する細菌株を含む組成物。
- エンテロコッカス・ガリナラム種の細菌株を含む、請求項1に記載の使用のための組成物。
- 細菌株が、配列番号3の少なくとも90%にわたり配列番号3と少なくとも95%の配列同一性を有する染色体を有する、請求項1又は2に記載の使用のための組成物。
- 肺がん、乳がん、肝臓がん又は結腸がんを治療又は予防する方法に使用するための、請求項1〜3のいずれかに記載の組成物。
- 腫瘍サイズを低減させる、腫瘍増殖を低減させる、転移を予防する、又は血管新生を予防する方法に使用するための、請求項1〜4のいずれかに記載の組成物。
- 細菌株が、エンテロコッカス・ガリナラムの細菌株の16s rRNA配列と少なくとも95%、96%、97%、98%、99%、99.5%又は99.9%同一である16s rRNA配列を有する、請求項1〜5のいずれかに記載の組成物。
- 細菌株が、配列番号1又は2と少なくとも95%、96%、97%、98%、99%、99.5%又は99.9%同一である16s rRNA配列を有する、請求項1〜6のいずれかに記載の組成物。
- 細菌株が、配列番号2と少なくとも95%、96%、97%、98%、99%、99.5%若しくは99.9%同一である16s rRNA配列を有するか、或いは
細菌株が、配列番号2によって表される16s rRNA配列を有する、
請求項7に記載の組成物。 - 経口投与用である、請求項1〜8のいずれかに記載の組成物。
- 1又は2以上の薬学的に許容される賦形剤又は担体を含む、請求項1〜9のいずれかに記載の組成物。
- 細菌株が凍結乾燥されている、請求項1〜10のいずれかに記載の組成物。
- 細菌株が生存しており、腸管に部分的又は全体的に定着することができる、請求項1〜11のいずれかに記載の組成物。
- エンテロコッカス・ガリナラムの単一株を含む、請求項1〜12のいずれかに記載の組成物。
- 微生物コンソーシアの一部としてエンテロコッカス・ガリナラム細菌株を含む、請求項1〜13のいずれかに記載の組成物。
- 請求項1〜5のいずれかに記載の使用のための、請求項1〜14のいずれかに記載の組成物を含む食品。
- 請求項1〜5のいずれかに記載の使用のための、請求項1〜14のいずれかに記載の組成物を含むワクチン組成物。
- がんを治療又は予防する方法であって、配列番号2と少なくとも95%同一である16s rRNA配列を有する細菌株を含む組成物を、それを必要とする患者に投与することを含む、前記方法。
- がんを治療又は予防する方法であって、それを必要とする患者にエンテロコッカス・ガリナラム種の細菌株を含む組成物を投与することを含む、前記方法。
- 受託番号NCIMB42488で寄託されたエンテロコッカス・ガリナラム株又はその派生物の細胞。
- 請求項19に記載の細胞を含む組成物。
- 薬学的に許容される担体又は賦形剤を含む、請求項20に記載の組成物。
- 受託番号NCIMB42488で寄託されたエンテロコッカス・ガリナラム株又はその派生物の生物学的に純粋な培養物。
- 治療に使用するための、受託番号NCIMB42488で寄託されたエンテロコッカス・ガリナラム株又はその派生物の細胞。
- 請求項1〜5のいずれかに規定の方法に使用するための、請求項23に記載の細胞。
- エンテロコッカス・ガリナラム種の1又は2以上の細菌株を含み、他の種の細菌を含有していない又はごく微量の若しくは生物学的に無関係な量の別の種の細菌のみを含む、治療に使用するための組成物。
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JP2021516216A (ja) * | 2018-01-19 | 2021-07-01 | フォーディー ファーマ リサーチ リミテッド4D Pharma Research Limited | がんを処置または予防するための併用療法 |
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