ES2626025T3 - Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas - Google Patents

Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas Download PDF

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ES2626025T3
ES2626025T3 ES13164585.5T ES13164585T ES2626025T3 ES 2626025 T3 ES2626025 T3 ES 2626025T3 ES 13164585 T ES13164585 T ES 13164585T ES 2626025 T3 ES2626025 T3 ES 2626025T3
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Homme W. Hellinga
James Jefferson Smith
Derek Jantz
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Abstract

Un método para escindir una secuencia de reconocimiento de diana de ADN bicatenario en una célula eucariota que comprende: introducir en dicha célula eucariota un ácido nucleico que codifica una meganucleasa; o una proteína meganucleasa; en el que dicha meganucleasa escinde dicha secuencia de reconocimiento de diana de ADN bicatenario; y en el que dicha meganucleasa es una meganucleasa recombinante que comprende: un polipéptido que tiene al menos un 85 % de similitud de secuencia con los restos 2-153 de la meganucleasa I-CreI de SEQ ID NO: 1; y que tiene especificidad por un semisitio de secuencia de reconocimiento que difiere en al menos un par de bases respecto de un semisitio en una secuencia de reconocimiento de meganucleasa I-CreI seleccionada entre el grupo que consiste en SEQ ID NO: 2, SEQ ID NO: 3, SEQ ID NO: 4 y SEQ ID NO: 5, en donde se ha alterado la especificidad en la posición -1: (i) a una A mediante una modificación seleccionada entre el grupo que consiste en D75C, D74L, D75Y, K139Y, T46A y T46C; (ii) a una G mediante una modificación seleccionada entre el grupo que consiste en T46E, T46D y T75E; o (iii) a una T mediante una modificación seleccionada entre el grupo que consiste en D75H, D75Q, D75Y, K139H, T46H y T46Q; (iv) a cualquier base en una hebra sentido mediante una modificación T46G. con la salvedad de que el método no es un método para el tratamiento del cuerpo humano o de un animal mediante terapia; con la salvedad de que el método no es un método para modificar la identidad genética de la línea germinal de seres humanos y con la salvedad adicional de que la célula no es una célula madre embrionaria humana o una célula de blastocisto humana.

Description

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Q46*
H46*
-2
Q70 E70 H70 Q44* C44*
T44*
D70 D44*
A44*
K44* E44*
V44*
R44*
I44*
L44*
N44*
-3
Q68 E68 R68 M68 H68 Y68 K68
C24*
F68 C68
I24*
K24* L68
R24*
F68
-4
A26* E77 R77 S77 S26*
Q77
K26* E26* Q26*
-5
E42 R42 K28* C28* M66
Q42
K66
-6
Q40 E40 R40 C40 A40 S40
C28*
R28* I40 A79 S28*
V40
A28*
C79
H28*
I79
V79
Q28*
-7
N30* E38 K38 I38 C38 H38
Q38
K30* R38 L38 N38
R30*
E30* Q30*
-8
F33 E33 F33 L33 R32* R33
Y33
D33 H33 V33
I33
F33
C33
-9
E32 R32 L32 D32 S32
K32
V32 132 N32
A32
H32
C32
Q32
T32
2.2.2 Meganucleasas recombinante específicamente excluidas
La presente invención no pretende adoptar ciertas meganucleasas recombinantes que se han descrito en la técnica
5 anterior y que se han desarrollado por métodos alternativos. Estas meganucleasas excluidas incluyen las descritas por Arnould et al (2006), J. Mol Biol. 355:443-58; Sussman et al (2004), J. Mol Biol. 342:31-41; Chames et al (2005), Nucleic Acids Res 33: e178; Seligman et al (2002), Nucleic Acids Res 30:3870-9; y Ashworth et al (2006), Nature 441 (7093): 656-659; las descripciones completas de las cuales se incorporan por la presente por referencia, incluyendo meganucleasas recombinantes basadas en I-CreI con sustituciones sencillas seleccionadas de C33,
10 R33, A44, H33, K32, F33, R32, A28, A70, E33, V33, A26 y R66. También se excluyen meganucleasas recombinantes basadas en I-CreI con tres sustituciones seleccionadas de A68/N70/N75 y D44/D70/N75, o con cuatro sustituciones seleccionadas de K44/T68/G60/N75 y R44/A68/T70/N75. Estas sustituciones o combinaciones de sustituciones se denominan en el presente documento “modificaciones excluidas”.
15 2.2.3 Meganucleasas con múltiples cambios en el semi-sitio de secuencia de reconocimiento
En otro aspecto, se describen meganucleasas diseñadas racionalmente que se producen combinando dos o más modificaciones de aminoácidos como se describe en la sección 2.2.1 anterior, para alterar la preferencia de semisitio en dos o más posiciones en un semi-sitio de secuencia de reconocimiento de ADN. Por ejemplo, sin limitación, 20 y como se describe más completamente posteriormente, la enzima DJ1 derivó de ICreI incorporando las modificaciones R30/E38 (que favorecen C en la posición -7), R40 (que favorece G en la posición -6), R42 (que favorece G en la posición -5) y N32 (que favorece degeneración completa en la posición -9). La meganucleasa DJ1 diseñada racionalmente reconoce de forma invariable C-7 G-6 G-5 en comparación con la preferencia de tipo
17
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como el promotor NOS, promotores génicos inducibles químicamente tales como el promotor inducible por dexametasona (véase, por ejemplo, Gremillon et al. (2004), Plant J. 37: 218-228), y promotores específicos de tejido vegetal tales como el promotor LGC1 (véase, por ejemplo, Singh et al. (2003), FEBS Lett. 542: 47-52).
5 Los métodos adecuados para introducir ADN en células vegetales incluyen prácticamente cualquier método por el que pueda introducirse ADN en una célula, incluyendo pero sin limitación una infección de Agrobacterium, transformación mediada por PEG de protoplastos (Omirulleh et al. (1993), Plant Molecular Biology, 21: 415-428), captación de ADN mediada por inhibición/desecación, electroporación, agitación con fibras de carburo de silicio, inyección balística o bombardeo de microproyectiles y similares.
En otras realizaciones, se produce un animal modificado genéticamente usando una meganucleasa recombinante. Como con células vegetales, las secuencias de ácido nucleico pueden introducirse en una célula germinal o una célula que con el tiempo se convertirá en un organismo transgénico, en el que dicha célula eucariota no es una célula madre humana o una célula de blastocisto humana. En algunas realizaciones, la célula es un huevo
15 fertilizado, y pueden inyectarse moléculas de ADN exógeno en el pro-núcleo del huevo fertilizado. Los huevos microinyectados se transfieren a los oviductos de madres adoptivas seudoembarazadas y se permite que se desarrollen. La meganucleasa recombinante se expresa en el huevo fertilizado (por ejemplo, bajo el control de un promotor constitutivo tal como 3-fosfoglicerato quinasa) y facilita la recombinación homóloga de la secuencia de interés en uno o varios sitios discretos en el genoma. Como alternativa, los animales modificados genéticamente pueden obtenerse utilizando células madre embrionarias recombinantes (“ES”) para la generación de los organismos transgénicos, como se describe en Gossler et al. (1986), Proc. Natl. Acad. Sci. USA 83: 9065 9069.
En ciertas realizaciones, un vector de expresión de mamíferos recombinante es capaz de dirigir la expresión específica de tejido del ácido nucleico preferentemente en un tipo celular particular. Se conocen en la técnica 25 elementos reguladores específicos de tejido. Los ejemplos no limitantes de promotores específicos de tejido adecuados incluyen el promotor de albúmina (específico de hígado; Pinkert et al. (1987), Genes Dev. 1: 268-277), promotores específicos linfoides (Calame y Eaton (1988), Adv. Immunol. 43: 235-275), en promotores particulares de receptores de linfocitos T (Winoto y Baltimore (1989), EMBO J. 8: 729-733) e inmunoglobulinas (Banerji et al. (1983), Cell 33: 729-740; Queen y Baltimore (1983), Cell 33: 741-748), promotores específicos de neuronas (por ejemplo, el promotor de neurofilamentos; Byrne y Ruddle (1989), Proc. Natl. Acad. Sci. USA 86: 5473-5477), promotores específicos del páncreas (Edlund et al. (1985), Science 230: 912-916) y promotores específicos de glándula mamaria (por ejemplo, promotor de suero de la leche; Patente de Estados Unidos N0 4.873.316 y Publicación de Patente Europea EP 0 264 166). También se abarcan promotores regulados por el desarrollo, por ejemplo, los promotores de hox murinos (Kessel y Gruss (1990), Science 249: 374-379) y el promotor de a-fetoproteína (Campes
35 y Tilghman (1989), Genes Dev. 3: 537-546).
En ciertas realizaciones, una meganucleasa diseñada racionalmente puede marcarse con un epítopo peptídico (por ejemplo, un epítopo HA, FLAG o Myc) para controlar los niveles de expresión o localización. En algunas realizaciones, la meganucleasa puede fusionarse con una señal de localización subcelular tal como una señal de localización nuclear (por ejemplo, la señal de localización nuclear de SV40) o señales de localización de cloroplastos
o mitocondrias. En otras realizaciones, la meganucleasa puede fusionarse con una señal de exportación nuclear para situarla en el citoplasma. La meganucleasa también puede fusionarse con una proteína no relacionada o dominio proteico tal como una proteína que estimula la recombinación homóloga o reparación de ADN (por ejemplo, recA, RAD51, RAD52, RAD54, RAD57 o BRCA2).
45
6. Métodos para Terapia Génica
Se describe el uso de meganucleasa recombinante para terapia génica. Como se usa en el presente documento, “terapia génica” significa tratamientos terapéuticos que comprenden introducir en un paciente una copia funcional de al menos un gen, o secuencia reguladora génica tal como un promotor, potenciador o silenciador para reemplazar un gen o región reguladora génica que sea defectuosa en su estructura y/o función. La expresión “terapia génica” también puede referirse a modificaciones hechas a un gen deletéreo o elemento regulador (por ejemplo, oncogenes) que reduce o elimina la expresión del gen. Puede realizarse terapia génica para tratar afecciones congénitas, afecciones resultantes de mutaciones o daño a loci genéticos específicos durante la vida del paciente, o afecciones
55 resultantes de organismos infecciosos.
En algunos aspectos, se reemplazan o deshabilitan genes disfuncionales mediante la inserción de secuencias de ácido nucleico exógeno en una región del genoma que afecta a la expresión génica. En ciertas realizaciones, la meganucleasa recombinante se dirige a una secuencia particular en la región del genoma para modificar de modo que alivie la afección. La secuencia puede ser una región dentro de un exón, intrón, promotor u otra región reguladora que esté provocando expresión disfuncional del gen. Como se usa en el presente documento, la expresión “expresión disfuncional” significa expresión aberrante de un producto génico porque la célula produce muy poco del producto génico, demasiado del producto génico, o produce un producto génico que tiene una función diferente tal como sin la función necesaria o que tiene más funciones que la necesaria.
65 Pueden usarse secuencias de ácido nucleico exógeno insertadas en la región modificada para proporcionar
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Claims (1)

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ES13164585.5T 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas Active ES2626025T3 (es)

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ES12162075.1T Active ES2440801T3 (es) 2005-10-18 2006-10-18 Meganucleasas racionalmente diseñadas con especificidad de secuencia y afinidad de unión a ADN alteradas
ES13164564.0T Active ES2602184T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
ES06826293T Active ES2425022T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
ES10191888T Active ES2384440T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
ES13164585.5T Active ES2626025T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
ES13164623.4T Active ES2539616T3 (es) 2005-10-18 2006-10-18 Meganucleasa diseñada racionalmente con afinidad de formación de dímeros alterada
ES17161899T Active ES2829549T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
ES13164628.3T Active ES2582091T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
ES10191904.1T Active ES2533370T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas

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ES06826293T Active ES2425022T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
ES10191888T Active ES2384440T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas

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ES13164628.3T Active ES2582091T3 (es) 2005-10-18 2006-10-18 Meganucleasas diseñadas racionalmente con especificidad de secuencia y afinidad de unión a ADN alteradas
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