Patent Application
20230201375
This disclosure relates to Neurofibromatosis Type I (NF1) as well as compositions and methods for using CRISPR/Cas-based systems to treat the same.
Neurofibromatosis Type I (NF1) is an autosomal dominant disease caused by the loss of function of the protein neurofibromin, a GTPase-activating protein that negatively regulates the Ras signaling pathway. Loss of neurofibromin leads to the formation of malignant and benign neurofibromas originating in non-dividing cells that form the myelin sheath of peripheral nerves, called Schwann cells. This disease affects 1 in 3,000 people worldwide, however, there is no effective treatment to reduce the size or number of neurofibromas. Gene editing technology could address the root cause of NF1 by correcting mutations in the NF1 gene, however, current approaches are not broadly applicable due to a series of limitations. First, the 8.6 kb NF1 coding sequence is too large to be delivered in its entirety via traditional gene therapy vectors. Second, no single patient mutation occurs in the population at a frequency greater than 2% and mutations are distributed along the full coding sequence of the gene, such that no single conventional gene editing approach can address a significant portion of the population. Finally, post-mitotic Schwann cells do not efficiently utilize homologous recombination pathways. Hence, there is still a great need for novel therapies and treatments for NF1.
In an aspect, the disclosure relates to a CRISPR/Cas-based genome editing system. The system may include (a) a polynucleotide sequence encoding a guide RNA (gRNA) targeting a fragment of a mutant NF1 gene; (b) a polynucleotide sequence encoding a Cas protein or a fusion protein comprising the Cas protein; and (c) a polynucleotide sequence encoding a donor sequence comprising a fragment of a wild-type NF1 gene. In some embodiments, the system comprises one or more vectors. In some embodiments, the system comprises a first vector and a second vector, wherein the first vector comprises the polynucleotide sequence encoding the gRNA, and the polynucleotide sequence encoding the Cas protein or the fusion protein, and the second vector comprises the polynucleotide sequence encoding the donor sequence. In some embodiments, the polynucleotide sequence encoding the gRNA and the polynucleotide sequence encoding the Cas protein or the fusion protein are operably linked. In some embodiments, the mutant NF1 gene comprises a mutation in the 5′ portion of the mutant NF1 gene, and the polynucleotide sequence encoding the donor sequence further comprises a stop codon that is 5′ to the donor sequence. In some embodiments, the gRNA targets a sequence upstream of the stop codon that is 5′ to the donor sequence and targets a sequence downstream of the donor sequence. In some embodiments, the polynucleotide sequence encoding the donor sequence further comprises a promoter in between the stop codon and the donor sequence. In some embodiments, the stop codon, the promoter, and the donor sequence are flanked on both ends (the 5′ and 3′ ends) with a sequence the gRNA targets. In some embodiments, the stop codon, the donor sequence, and the 3′ portion of the mutant NF1 gene are in the same reading frame. In some embodiments, the mutant NF1 gene comprises a mutation in the 3′ portion of the mutant NF1 gene, and the polynucleotide sequence encoding the donor sequence further comprises a stop codon that is 3′ to the donor sequence. In some embodiments, the gRNA targets a sequence upstream of the donor sequence and targets a sequence downstream of the stop codon that is 3′ to the donor sequence. In some embodiments, the 5′ portion of the mutant NF1 gene, the donor sequence, and the stop codon are in the same reading frame. In some embodiments, the gRNA targets a sequence flanking both sides of the polynucleotide sequence encoding the donor sequence and the stop codon. In some embodiments, the donor sequence comprises multiple exons of the wild-type NF1 gene or a functional equivalent thereof. In some embodiments, the donor sequence comprises one or more exons selected from exon 1, exon 2, exon 3, exon 4, exon 5, exon 6, exon 7, exon 8, exon 9, exon 10, exon 11, exon 12, exon 13, exon 14, exon 15, exon 16, exon 17, exon 18, exon 19, exon 20, exon 21, exon 22, exon 23, exon 24, exon 25, exon 26, exon 27, exon 28, exon 29, exon 30, exon 31, exon 32, exon 33, exon 34, exon 35, exon 36, exon 37, exon 38, exon 39, exon 40, exon 41, exon 42, exon 43, exon 44, exon 45, exon 46, exon 47, exon 48, exon 49, exon 50, exon 51, exon 52, exon 53, exon 54, exon 55, exon 56, and exon 57 of the wild-type NF1 gene or a functional equivalent thereof. In some embodiments, the donor sequence comprises one or more contiguous exons of the wild-type NF1 gene or a functional equivalent thereof. In some embodiments, the donor sequence comprises exons 1-30 of the wild-type NF1 gene, and the gRNA targets a fragment of a mutant NF1 gene between exon 30 and exon 31. In some embodiments, the gRNA comprises a polynucleotide sequence selected from SEQ ID NOs: 71-81 or a complement thereof or a truncation thereof. In some embodiments, the gRNA is encoded by a polynucleotide sequence selected from SEQ ID NOs: 60-70 or a complement thereof or a truncation thereof, and/or hybridizes to a polynucleotide sequence selected from SEQ ID NOs: 49-59 or a complement thereof or a truncation thereof. In some embodiments, the donor sequence comprises a polynucleotide sequence of SEQ ID NO: 82. In some embodiments, the Cas protein is a Streptococcus pyogenes Cas9 protein or a Staphylococcus aureus Cas9 protein. In some embodiments, the Cas protein comprises an amino acid sequence of SEQ ID NO: 20 or SEQ ID NO: 21. In some embodiments, the vector is a viral vector. In some embodiments, the vector is an Adeno-associated virus (AAV) vector. In some embodiments, the AAV vector is AAV1, AAV2, AAV3, AAV4, AAV5, AAV6, AAV7, AAV8, AAV9, AAV-10, AAV-11, AAV-12, AAV-13, or AAVrh.74 vector. In some embodiments, one of the one or more vectors comprises a polynucleotide sequence selected from SEQ ID NOs: 83-102. In some embodiments, the molar ratio between the gRNA and the donor sequence is 1:1, or 1:5, or from 5:1 to 1:10, or from 1:1 to 1:5.
In a further aspect, the disclosure relates to a cell comprising a system as detailed herein.
Another aspect of the disclosure provides a composition for restoring NF1 function in a cell having a mutant NF1 gene, the composition comprising a system as detailed herein or a cell as detailed herein.
Another aspect of the disclosure provides a kit comprising a system as detailed herein, a cell as detailed herein, or a composition as detailed herein.
Another aspect of the disclosure provides a method for restoring NF1 function in a cell or a subject having a mutant NF1 gene. The method may include contacting the cell or the subject with a system as detailed herein, a cell as detailed herein, or a composition as detailed herein. In some embodiments, NF1 function is restored by inserting one or more wild-type exons of NF1 gene corresponding to the mutant NF1 gene.
The disclosure provides for other aspects and embodiments that will be apparent in light of the following detailed description and accompanying figures.
Provided herein are systems and methods that utilize a CRISPR/Cas-based strategy to restore the correct NF1 gene sequence, for example, through the nonhomologous end joining repair process in a subject suffering from NF1. The CRISPR/Cas-based genome editing systems detailed herein may include a polynucleotide sequence encoding a guide RNA (gRNA) targeting a fragment of a mutant NF1 gene, a polynucleotide sequence encoding a Cas protein or a fusion protein comprising the Cas protein, and a polynucleotide sequence encoding a donor sequence comprising a fragment of a wild-type NF1 gene. The systems may be used in compositions, kits, and methods for restoring NF1 function and/or treating Neurofibromatosis Type I (NF1). In some embodiments, the systems and methods comprise the delivery of one or two ~5 kb donor cassettes or vectors, encoding either the 5′ or the 3′ portion of the NF1 cDNA sequence, depending on the patient mutation, flanked by a S. aureus Cas9 (SaCas9) guide RNA (gRNA) target site that corresponds to a sequence in a middle portion of the NF1 gene. For mutations occurring in either the 5′ or the 3′ portion of the gene, the corresponding donor would be used. Co-delivery of SaCas9 and the gRNA with the appropriate donor leads to a double-strand break in the middle portion of the NF1 gene and on both sides of the donor sequence, creating free DNA ends for ligation of the donor sequence into the genomic double-strand break, thereby restoring a wild-type NF1 coding sequence. The systems and methods provided herein result in the production of functional neurofibromin and lead to a reduction in Ras signaling and a decrease in the size and number of tumors in a NF1 mouse model. Further provided herein are methods of treating a subject suffering from, or at risk of developing, NF1 using the systems and methods provided herein. The systems and methods provided herein are estimated to be applicable to over 90% of NF1 patients.
The compositions and methods detailed herein have several advantages over conventional gene replacement and gene editing approaches. For example, the compositions and methods detailed herein include the ability for the gene to be regulated by endogenous machinery, and the ability to correct a large portion of the mutations in the patient population with a single donor sequence. Additionally, for diseases like NF1 that lack a prevalent mutation or a hot spot, the compositions and methods detailed here provide a viable strategy to treat a significant portion of the patient population.
Unless otherwise defined, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art. In case of conflict, the present document, including definitions, will control. Preferred methods and materials are described below, although methods and materials similar or equivalent to those described herein can be used in practice or testing of the present invention. All publications, patent applications, patents and other references mentioned herein are incorporated by reference in their entirety. The materials, methods, and examples disclosed herein are illustrative only and not intended to be limiting.
The terms “comprise(s),” “include(s),” “having,” “has,” “can,” “contain(s),” and variants thereof, as used herein, are intended to be open-ended transitional phrases, terms, or words that do not preclude the possibility of additional acts or structures. The singular forms “a,” “and,” and “the” include plural references unless the context clearly dictates otherwise. The present disclosure also contemplates other embodiments “comprising,” “consisting of,” and “consisting essentially of,” the embodiments or elements presented herein, whether explicitly set forth or not.
For the recitation of numeric ranges herein, each intervening number there between with the same degree of precision is explicitly contemplated. For example, for the range of 6-9, the numbers 7 and 8 are contemplated in addition to 6 and 9, and for the range 6.0-7.0, the number 6.0, 6.1, 6.2, 6.3, 6.4, 6.5, 6.6, 6.7, 6.8, 6.9, and 7.0 are explicitly contemplated.
The term “about” or “approximately” as used herein as applied to one or more values of interest, refers to a value that is similar to a stated reference value, or within an acceptable error range for the particular value as determined by one of ordinary skill in the art, which will depend in part on how the value is measured or determined, such as the limitations of the measurement system. In certain aspects, the term “about” refers to a range of values that fall within 20%, 19%, 18%, 17%, 16%, 15%, 14%, 13%, 12%, 11%, 10%, 9%, 8%, 7%, 6%, 5%, 4%, 3%, 2%, 1%, or less in either direction (greater than or less than) of the stated reference value unless otherwise stated or otherwise evident from the context (except where such number would exceed 100% of a possible value). Alternatively, “about” can mean within 3 or more than 3 standard deviations, per the practice in the art. Alternatively, such as with respect to biological systems or processes, the term “about” can mean within an order of magnitude, preferably within 5-fold, and more preferably within 2-fold, of a value.
“Adeno-associated virus” or “AAV” as used interchangeably herein refers to a small virus belonging to the genus Dependovirus of the Parvoviridae family that infects humans and some other primate species. AAV is not currently known to cause disease and consequently the virus causes a very mild immune response.
“Amino acid” as used herein refers to naturally occurring and non-natural synthetic amino acids, as well as amino acid analogs and amino acid mimetics that function in a manner similar to the naturally occurring amino acids. Naturally occurring amino acids are those encoded by the genetic code. Amino acids can be referred to herein by either their commonly known three-letter symbols or by the one-letter symbols recommended by the IUPAC-IUB Biochemical Nomenclature Commission. Amino acids include the side chain and polypeptide backbone portions.
“Binding region” as used herein refers to the region within a target region that is recognized and bound by the CRISPR/Cas-based gene editing system.
“Clustered Regularly Interspaced Short Palindromic Repeats” and “CRISPRs”, as used interchangeably herein, refers to loci containing multiple short direct repeats that are found in the genomes of approximately 40% of sequenced bacteria and 90% of sequenced archaea.
“Coding sequence” or “encoding nucleic acid” as used herein means the nucleic acids (RNA or DNA molecule) that comprise a nucleotide sequence which encodes a protein. The coding sequence can further include initiation and termination signals operably linked to regulatory elements including a promoter and polyadenylation signal capable of directing expression in the cells of an individual or mammal to which the nucleic acid is administered. The regulatory elements may include, for example, a promoter, an enhancer, an initiation codon, a stop codon, or a polyadenylation signal. The coding sequence may be codon optimized.
“Complement” or “complementary” as used herein means a nucleic acid can mean Watson-Crick (e.g., A-T/U and C-G) or Hoogsteen base pairing between nucleotides or nucleotide analogs of nucleic acid molecules. “Complementarity” refers to a property shared between two nucleic acid sequences, such that when they are aligned antiparallel to each other, the nucleotide bases at each position will be complementary.
The terms “control,” “reference level,” and “reference” are used herein interchangeably. The reference level may be a predetermined value or range, which is employed as a benchmark against which to assess the measured result. “Control group” as used herein refers to a group of control subjects. The predetermined level may be a cutoff value from a control group. The predetermined level may be an average from a control group. Cutoff values (or predetermined cutoff values) may be determined by Adaptive Index Model (AIM) methodology. Cutoff values (or predetermined cutoff values) may be determined by a receiver operating curve (ROC) analysis from biological samples of the patient group. ROC analysis, as generally known in the biological arts, is a determination of the ability of a test to discriminate one condition from another, e.g., to determine the performance of each marker in identifying a patient having CRC. A description of ROC analysis is provided in P.J. Heagerty et al. (Biometrics 2000, 56, 337-44), the disclosure of which is hereby incorporated by reference in its entirety. Alternatively, cutoff values may be determined by a quartile analysis of biological samples of a patient group. For example, a cutoff value may be determined by selecting a value that corresponds to any value in the 25th-75th percentile range, preferably a value that corresponds to the 25th percentile, the 50th percentile or the 75th percentile, and more preferably the 75th percentile. Such statistical analyses may be performed using any method known in the art and can be implemented through any number of commercially available software packages (e.g., from Analyse-it Software Ltd., Leeds, UK; StataCorp LP, College Station, TX; SAS Institute Inc., Cary, NC.). The healthy or normal levels or ranges for a target or for a protein activity may be defined in accordance with standard practice. A control may be a subject or cell without a composition as detailed herein. A control may be a subject, or a sample therefrom, whose disease state is known. The subject, or sample therefrom, may be healthy, diseased, diseased prior to treatment, diseased during treatment, or diseased after treatment, or a combination thereof.
“Correcting”, “gene editing,” and “restoring” as used herein refers to changing a mutant gene that encodes a dysfunctional protein or truncated protein or no protein at all, such that a full-length functional or partially full-length functional protein expression is obtained. Correcting or restoring a mutant gene may include replacing the region of the gene that has the mutation or replacing the entire mutant gene with a copy of the gene that does not have the mutation with a repair mechanism such as homology-directed repair (HDR). Correcting or restoring a mutant gene may also include repairing a frameshift mutation that causes a premature stop codon, an aberrant splice acceptor site or an aberrant splice donor site, by generating a double stranded break in the gene that is then repaired using non-homologous end joining (NHEJ). NHEJ may add or delete at least one base pair during repair which may restore the proper reading frame and eliminate the premature stop codon. Correcting or restoring a mutant gene may also include disrupting an aberrant splice acceptor site or splice donor sequence. Correcting or restoring a mutant gene may also include deleting a non-essential gene segment by the simultaneous action of two nucleases on the same DNA strand in order to restore the proper reading frame by removing the DNA between the two nuclease target sites and repairing the DNA break by NHEJ.
“Donor DNA”, “donor template,” and “repair template” as used interchangeably herein refers to a double-stranded DNA fragment or molecule that includes at least a portion of the gene of interest. The donor DNA may encode a full-functional protein or a partially functional protein.
“Enhancer” as used herein refers to non-coding DNA sequences containing multiple activator and repressor binding sites. Enhancers range from 200 bp to 1 kb in length and may be either proximal, 5′ upstream to the promoter or within the first intron of the regulated gene, or distal, in introns of neighboring genes or intergenic regions far away from the locus. Through DNA looping, active enhancers contact the promoter dependently of the core DNA binding motif promoter specificity. 4 to 5 enhancers may interact with a promoter. Similarly, enhancers may regulate more than one gene without linkage restriction and may “skip” neighboring genes to regulate more distant ones. Transcriptional regulation may involve elements located in a chromosome different to one where the promoter resides. Proximal enhancers or promoters of neighboring genes may serve as platforms to recruit more distal elements.
“Frameshift” or “frameshift mutation” as used interchangeably herein refers to a type of gene mutation wherein the addition or deletion of one or more nucleotides causes a shift in the reading frame of the codons in the mRNA. The shift in reading frame may lead to the alteration in the amino acid sequence at protein translation, such as a missense mutation or a premature stop codon.
“Functional” and “full-functional” as used herein describes protein that has biological activity. A “functional gene” refers to a gene transcribed to mRNA, which is translated to a functional protein.
“Fusion protein” as used herein refers to a chimeric protein created through the joining of two or more genes that originally coded for separate proteins. The translation of the fusion gene results in a single polypeptide with functional properties derived from each of the original proteins.
“Genetic construct” as used herein refers to the DNA or RNA molecules that comprise a polynucleotide that encodes a protein. The coding sequence includes initiation and termination signals operably linked to regulatory elements including a promoter and polyadenylation signal capable of directing expression in the cells of the individual to whom the nucleic acid molecule is administered. As used herein, the term “expressible form” refers to gene constructs that contain the necessary regulatory elements operable linked to a coding sequence that encodes a protein such that when present in the cell of the individual, the coding sequence will be expressed. The regulatory elements may include, for example, a promoter, an enhancer, an initiation codon, a stop codon, or a polyadenylation signal.
“Genome editing” or “gene editing” as used herein refers to changing the DNA sequence of a gene. Genome editing may include correcting or restoring a mutant gene or adding additional mutations. Genome editing may include knocking out a gene, such as a mutant gene or a normal gene. Genome editing may be used to treat disease or, for example, enhance muscle repair, by changing the gene of interest. In some embodiments, the compositions and methods detailed herein are for use in somatic cells and not germ line cells.
The term “heterologous” as used herein refers to nucleic acid comprising two or more subsequences that are not found in the same relationship to each other in nature. For instance, a nucleic acid that is recombinantly produced typically has two or more sequences from unrelated genes synthetically arranged to make a new functional nucleic acid, for example, a promoter from one source and a coding region from another source. The two nucleic acids are thus heterologous to each other in this context. When added to a cell, the recombinant nucleic acids would also be heterologous to the endogenous genes of the cell. Thus, in a chromosome, a heterologous nucleic acid would include a non-native (non-naturally occurring) nucleic acid that has integrated into the chromosome, or a non-native (non-naturally occurring) extrachromosomal nucleic acid. Similarly, a heterologous protein indicates that the protein comprises two or more subsequences that are not found in the same relationship to each other in nature (for example, a “fusion protein,” where the two subsequences are encoded by a single nucleic acid sequence).
“Homology-directed repair” or “HDR” as used interchangeably herein refers to a mechanism in cells to repair double strand DNA lesions when a homologous piece of DNA is present in the nucleus, mostly in G2 and S phase of the cell cycle. HDR uses a donor DNA template to guide repair and may be used to create specific sequence changes to the genome, including the targeted addition of whole genes. If a donor template is provided along with the CRISPR/Cas-based gene editing system, then the cellular machinery will repair the break by homologous recombination, which is enhanced several orders of magnitude in the presence of DNA cleavage. When the homologous DNA piece is absent, non-homologous end joining may take place instead.
“Identical” or “identity” as used herein in the context of two or more polynucleotide or polypeptide sequences means that the sequences have a specified percentage of residues that are the same over a specified region. The percentage may be calculated by optimally aligning the two sequences, comparing the two sequences over the specified region, determining the number of positions at which the identical residue occurs in both sequences to yield the number of matched positions, dividing the number of matched positions by the total number of positions in the specified region, and multiplying the result by 100 to yield the percentage of sequence identity. In cases where the two sequences are of different lengths or the alignment produces one or more staggered ends and the specified region of comparison includes only a single sequence, the residues of single sequence are included in the denominator but not the numerator of the calculation. When comparing DNA and RNA, thymine (T) and uracil (U) may be considered equivalent. Identity may be performed manually or by using a computer sequence algorithm such as BLAST or BLAST 2.0.
“Mutant gene” or “mutated gene” as used interchangeably herein refers to a gene that has undergone a detectable mutation. A mutant gene has undergone a change, such as the loss, gain, or exchange of genetic material, which affects the normal transmission and expression of the gene. A “disrupted gene” as used herein refers to a mutant gene that has a mutation that causes a premature stop codon. The disrupted gene product is truncated relative to a full-length undisrupted gene product.
“Non-homologous end joining (NHEJ) pathway” as used herein refers to a pathway that repairs double-strand breaks in DNA by directly ligating the break ends without the need for a homologous template. The template-independent re-ligation of DNA ends by NHEJ is a stochastic, error-prone repair process that introduces random micro-insertions and micro-deletions (indels) at the DNA breakpoint. This method may be used to intentionally disrupt, delete, or alter the reading frame of targeted gene sequences. NHEJ typically uses short homologous DNA sequences called microhomologies to guide repair. These microhomologies are often present in single-stranded overhangs on the end of double-strand breaks. When the overhangs are perfectly compatible, NHEJ usually repairs the break accurately, yet imprecise repair leading to loss of nucleotides may also occur, but is much more common when the overhangs are not compatible. “Nuclease mediated NHEJ” as used herein refers to NHEJ that is initiated after a nuclease cuts double stranded DNA.
“Normal gene” as used herein refers to a gene that has not undergone a change, such as a loss, gain, or exchange of genetic material. The normal gene undergoes normal gene transmission and gene expression. For example, a normal gene may be a wild-type gene.
“Nucleic acid” or “oligonucleotide” or “polynucleotide” as used herein means at least two nucleotides covalently linked together. The depiction of a single strand also defines the sequence of the complementary strand. Thus, a polynucleotide also encompasses the complementary strand of a depicted single strand. Many variants of a polynucleotide may be used for the same purpose as a given polynucleotide. Thus, a polynucleotide also encompasses substantially identical polynucleotides and complements thereof. A single strand provides a probe that may hybridize to a target sequence under stringent hybridization conditions. Thus, a polynucleotide also encompasses a probe that hybridizes under stringent hybridization conditions. Polynucleotides may be single stranded or double stranded or may contain portions of both double stranded and single stranded sequence. The polynucleotide can be nucleic acid, natural or synthetic, DNA, genomic DNA, cDNA, RNA, or a hybrid, where the polynucleotide can contain combinations of deoxyribo-and ribo-nucleotides, and combinations of bases including, for example, uracil, adenine, thymine, cytosine, guanine, inosine, xanthine hypoxanthine, isocytosine, and isoguanine. Polynucleotides can be obtained by chemical synthesis methods or by recombinant methods.
“Open reading frame” refers to a stretch of codons that begins with a start codon and ends at a stop codon. In eukaryotic genes with multiple exons, introns are removed, and exons are then joined together after transcription to yield the final mRNA for protein translation. An open reading frame may be a continuous stretch of codons. In some embodiments, the open reading frame only applies to spliced mRNAs, not genomic DNA, for expression of a protein.
“Operably linked” as used herein means that expression of a gene is under the control of a promoter with which it is spatially connected. A promoter may be positioned 5′ (upstream) or 3′ (downstream) of a gene under its control. The distance between the promoter and a gene may be approximately the same as the distance between that promoter and the gene it controls in the gene from which the promoter is derived. As is known in the art, variation in this distance may be accommodated without loss of promoter function. Nucleic acid or amino acid sequences are “operably linked” (or “operatively linked”) when placed into a functional relationship with one another. For instance, a promoter or enhancer is operably linked to a coding sequence if it regulates, or contributes to the modulation of, the transcription of the coding sequence. Operably linked DNA sequences are typically contiguous, and operably linked amino acid sequences are typically contiguous and in the same reading frame. However, since enhancers generally function when separated from the promoter by up to several kilobases or more and intronic sequences may be of variable lengths, some polynucleotide elements may be operably linked but not contiguous. Similarly, certain amino acid sequences that are non-contiguous in a primary polypeptide sequence may nonetheless be operably linked due to, for example folding of a polypeptide chain. With respect to fusion polypeptides, the terms “operatively linked” and “operably linked” can refer to the fact that each of the components performs the same function in linkage to the other component as it would if it were not so linked.
“Partially-functional” as used herein describes a protein that is encoded by a mutant gene and has less biological activity than a functional protein but more than a non-functional protein.
A “peptide” or “polypeptide” is a linked sequence of two or more amino acids linked by peptide bonds. The polypeptide can be natural, synthetic, or a modification or combination of natural and synthetic. Peptides and polypeptides include proteins such as binding proteins, receptors, and antibodies. The terms “polypeptide”, “protein,” and “peptide” are used interchangeably herein. “Primary structure” refers to the amino acid sequence of a particular peptide. “Secondary structure” refers to locally ordered, three dimensional structures within a polypeptide. These structures are commonly known as domains, for example, enzymatic domains, extracellular domains, transmembrane domains, pore domains, and cytoplasmic tail domains. “Domains” are portions of a polypeptide that form a compact unit of the polypeptide and are typically 15 to 350 amino acids long. Exemplary domains include domains with enzymatic activity or ligand binding activity. Typical domains are made up of sections of lesser organization such as stretches of beta-sheet and alpha-helices. “Tertiary structure” refers to the complete three-dimensional structure of a polypeptide monomer. “Quaternary structure” refers to the three-dimensional structure formed by the noncovalent association of independent tertiary units. A “motif” is a portion of a polypeptide sequence and includes at least two amino acids. A motif may be 2 to 20, 2 to 15, or 2 to 10 amino acids in length. In some embodiments, a motif includes 3, 4, 5, 6, or 7 sequential amino acids. A domain may be comprised of a series of the same type of motif.
“Premature stop codon” or “out-of-frame stop codon” as used interchangeably herein refers to nonsense mutation in a sequence of DNA, which results in a stop codon at location not normally found in the wild-type gene. A premature stop codon may cause a protein to be truncated or shorter compared to the full-length version of the protein.
“Promoter” as used herein means a synthetic or naturally derived molecule which is capable of conferring, activating or enhancing expression of a nucleic acid in a cell. A promoter may comprise one or more specific transcriptional regulatory sequences to further enhance expression and/or to alter the spatial expression and/or temporal expression of same. A promoter may also comprise distal enhancer or repressor elements, which may be located as much as several thousand base pairs from the start site of transcription. A promoter may be derived from sources including viral, bacterial, fungal, plants, insects, and animals. A promoter may regulate the expression of a gene component constitutively, or differentially with respect to cell, the tissue or organ in which expression occurs or, with respect to the developmental stage at which expression occurs, or in response to external stimuli such as physiological stresses, pathogens, metal ions, or inducing agents. Representative examples of promoters include the bacteriophage T7 promoter, bacteriophage T3 promoter, SP6 promoter, lac operator-promoter, tac promoter, SV40 late promoter, SV40 early promoter, RSV-LTR promoter, CMV IE promoter, SV40 early promoter or SV40 late promoter, human U6 (hU6) promoter, and CMV IE promoter. Promoters that target muscle-specific stem cells may include the CK8 promoter, the Spc5-12 promoter, and the MHCK7 promoter.
The term “recombinant” when used with reference to, for example, a cell, nucleic acid, protein, or vector, indicates that the cell, nucleic acid, protein, or vector, has been modified by the introduction of a heterologous nucleic acid or protein or the alteration of a native nucleic acid or protein, or that the cell is derived from a cell so modified. Thus, for example, recombinant cells express genes that are not found within the native (naturally occurring) form of the cell or express a second copy of a native gene that is otherwise normally or abnormally expressed, under expressed, or not expressed at all.
“Sample” or “test sample” as used herein can mean any sample in which the presence and/or level of a target is to be detected or determined or any sample comprising a DNA targeting or gene editing system or component thereof as detailed herein. Samples may include liquids, solutions, emulsions, or suspensions. Samples may include a medical sample. Samples may include any biological fluid or tissue, such as blood, whole blood, fractions of blood such as plasma and serum, muscle, interstitial fluid, sweat, saliva, urine, tears, synovial fluid, bone marrow, cerebrospinal fluid, nasal secretions, sputum, amniotic fluid, bronchoalveolar lavage fluid, gastric lavage, emesis, fecal matter, lung tissue, peripheral blood mononuclear cells, total white blood cells, lymph node cells, spleen cells, tonsil cells, cancer cells, tumor cells, bile, digestive fluid, skin, or combinations thereof. In some embodiments, the sample comprises an aliquot. In other embodiments, the sample comprises a biological fluid. Samples can be obtained by any means known in the art. The sample can be used directly as obtained from a patient or can be pre-treated, such as by filtration, distillation, extraction, concentration, centrifugation, inactivation of interfering components, addition of reagents, and the like, to modify the character of the sample in some manner as discussed herein or otherwise as is known in the art.
“Subject” and “patient” as used herein interchangeably refers to any vertebrate, including, but not limited to, a mammal that wants or is in need of the herein described compositions or methods. The subject may be a human or a non-human. The subject may be a vertebrate. The subject may be a mammal. The mammal may be a primate or a non-primate. The mammal can be a non-primate such as, for example, cow, pig, camel, llama, hedgehog, anteater, platypus, elephant, alpaca, horse, goat, rabbit, sheep, hamster, guinea pig, cat, dog, rat, and mouse. The mammal can be a primate such as a human. The mammal can be a non-human primate such as, for example, monkey, cynomolgous monkey, rhesus monkey, chimpanzee, gorilla, orangutan, and gibbon. The subject may be of any age or stage of development, such as, for example, an adult, an adolescent, a child, such as age 0-2, 2-4, 2-6, or 6-12 years, or an infant, such as age 0-1 years. The subject may be male. The subject may be female. In some embodiments, the subject has a specific genetic marker. The subject may be undergoing other forms of treatment.
“Substantially identical” can mean that a first and second amino acid or polynucleotide sequence are at least 60%, 65%, 70%, 75%, 80%, 85%, 90%, 95%, 96%, 97%, 98%, or 99% over a region of 1, 2, 3, 4, 5, 6, 7, 8, 9, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, 20, 21, 22, 23, 24, 25, 30, 35, 40, 45, 50, 55, 60, 65, 70, 75, 80, 85, 90, 95, 100, 200, 300, 400, 500, 600, 700, 800, 900, 1000, 1100 amino acids or nucleotides, respectively.
“Target gene” as used herein refers to any nucleotide sequence encoding a known or putative gene product. The target gene may be a mutated gene involved in a genetic disease. The target gene may encode a known or putative gene product that is intended to be corrected or for which its expression is intended to be modulated. In certain embodiments, the target gene is the NF1 gene.
“Target region” as used herein refers to the region of the target gene to which the CRISPR/Cas-based gene editing or targeting system is designed to bind. In some embodiments, the target region is within an intronic region between exon 30 and exon 31 of the NF1 gene.
“Transgene” as used herein refers to a gene or genetic material containing a gene sequence that has been isolated from one organism and is introduced into a different organism. This non-native segment of DNA may retain the ability to produce RNA or protein in the transgenic organism, or it may alter the normal function of the transgenic organism’s genetic code. The introduction of a transgene has the potential to change the phenotype of an organism.
“Transcriptional regulatory elements” or “regulatory elements” refers to a genetic element which can control the expression of nucleic acid sequences, such as activate, enhancer, or decrease expression, or alter the spatial and/or temporal expression of a nucleic acid sequence. Examples of regulatory elements include, for example, promoters, enhancers, splicing signals, polyadenylation signals, and termination signals. A regulatory element can be “endogenous,” “exogenous,” or “heterologous” with respect to the gene to which it is operably linked. An “endogenous” regulatory element is one which is naturally linked with a given gene in the genome. An “exogenous” or “heterologous” regulatory element is one which is not normally linked with a given gene but is placed in operable linkage with a gene by genetic manipulation.
“Treatment” or “treating” or “therapy” when referring to protection of a subject from a disease, means suppressing, repressing, reversing, alleviating, ameliorating, or inhibiting the progress of disease, or completely eliminating a disease. A treatment may be either performed in an acute or chronic way. The term also refers to reducing the severity of a disease or symptoms associated with such disease prior to affliction with the disease. Treatment may result in a reduction in the incidence, frequency, severity, and/or duration of symptoms of the disease. Preventing the disease involves administering a composition of the present invention to a subject prior to onset of the disease. Suppressing the disease involves administering a composition of the present invention to a subject after induction of the disease but before its clinical appearance. Repressing or ameliorating the disease involves administering a composition of the present invention to a subject after clinical appearance of the disease.
As used herein, the term “gene therapy” refers to a method of treating a patient wherein polypeptides or nucleic acid sequences are transferred into cells of a patient such that activity and/or the expression of a particular gene is modulated. In certain embodiments, the expression of the gene is suppressed. In certain embodiments, the expression of the gene is enhanced. In certain embodiments, the temporal or spatial pattern of the expression of the gene is modulated.
“Variant” used herein with respect to a polynucleotide means (i) a portion or fragment of a referenced nucleotide sequence; (ii) the complement of a referenced nucleotide sequence or portion thereof; (iii) a nucleic acid that is substantially identical to a referenced nucleic acid or the complement thereof; or (iv) a nucleic acid that hybridizes under stringent conditions to the referenced nucleic acid, complement thereof, or a sequences substantially identical thereto.
“Variant” with respect to a peptide or polypeptide that differs in amino acid sequence by the insertion, deletion, or conservative substitution of amino acids, but retain at least one biological activity. Variant may also mean a protein with an amino acid sequence that is substantially identical to a referenced protein with an amino acid sequence that retains at least one biological activity. Representative examples of “biological activity” include the ability to be bound by a specific antibody or polypeptide or to promote an immune response. Variant can mean a functional fragment thereof. Variant can also mean multiple copies of a polypeptide. The multiple copies can be in tandem or separated by a linker. A conservative substitution of an amino acid, for example, replacing an amino acid with a different amino acid of similar properties (for example, hydrophilicity, degree and distribution of charged regions) is recognized in the art as typically involving a minor change. These minor changes may be identified, in part, by considering the hydropathic index of amino acids, as understood in the art (Kyte et al., J. Mol. Biol. 1982, 157, 105-132). The hydropathic index of an amino acid is based on a consideration of its hydrophobicity and charge. It is known in the art that amino acids of similar hydropathic indexes may be substituted and still retain protein function. In one aspect, amino acids having hydropathic indexes of ±2 are substituted. The hydrophilicity of amino acids may also be used to reveal substitutions that would result in proteins retaining biological function. A consideration of the hydrophilicity of amino acids in the context of a peptide permits calculation of the greatest local average hydrophilicity of that peptide. Substitutions may be performed with amino acids having hydrophilicity values within ±2 of each other. Both the hydrophobicity index and the hydrophilicity value of amino acids are influenced by the particular side chain of that amino acid. Consistent with that observation, amino acid substitutions that are compatible with biological function are understood to depend on the relative similarity of the amino acids, and particularly the side chains of those amino acids, as revealed by the hydrophobicity, hydrophilicity, charge, size, and other properties.
“Vector” as used herein means a nucleic acid sequence containing an origin of replication. A vector may be capable of directing the delivery or transfer of a polynucleotide sequence to target cells, where it can be replicated or expressed. A vector may contain an origin of replication, one or more regulatory elements, and/or one or more coding sequences. A vector may be a viral vector, bacteriophage, bacterial artificial chromosome, plasmid, cosmid, or yeast artificial chromosome. A vector may be a DNA or RNA vector. A vector may be a self-replicating extrachromosomal vector. Viral vectors include, but are not limited to, adenovirus vector, adeno-associated virus (AAV) vector, retrovirus vector, or lentivirus vector. A vector may be an adeno-associated virus (AAV) vector. The vector may encode a Cas9 protein and at least one gRNA molecule.
Unless otherwise defined herein, scientific and technical terms used in connection with the present disclosure shall have the meanings that are commonly understood by those of ordinary skill in the art. For example, any nomenclatures used in connection with, and techniques of, cell and tissue culture, molecular biology, immunology, microbiology, genetics, and protein and nucleic acid chemistry and hybridization described herein are those that are well known and commonly used in the art. The meaning and scope of the terms should be clear; in the event however of any latent ambiguity, definitions provided herein take precedent over any dictionary or extrinsic definition. Further, unless otherwise required by context, singular terms shall include pluralities and plural terms shall include the singular.
Neurofibromatosis Type I (NF1; also known as von Recklinghausen syndrome) is an autosomal dominant disease caused by the loss of function of the protein neurofibromin (which may also be referred to a NF1). Loss of neurofibromin leads to the formation of malignant and benign neurofibromas originating in non-dividing cells that form the myelin sheath of peripheral nerves, called Schwann cells. Additional symptoms of NF1 may include disfiguring cutaneous neurofibromas (CNF), café au lait pigment spots, plexiform neurofibromas (PN), skeletal defects, optic nerve gliomas, life-threatening malignant peripheral nerve sheath tumors (MPNST), pheochromocytoma, attention deficits, learning deficits, and other cognitive disabilities. NF1 affects 1 in 3,000 people worldwide, however, there is currently no effective treatment to reduce the size or number of neurofibromas.
Neurofibromin is a GTPase-activating protein (GAP) that negatively regulates RAS/MAPK cellular growth and proliferation pathway activity by accelerating the hydrolysis of Ras-bound GTP. Neurofibromin primarily regulates the protein Ras. Human neurofibromin is a 320-kDa protein that includes 2,818 amino acids. Neurofibromin localizes in the cytoplasm, however, some studies have found neurofibromin or fragments of it in the nucleus. Neurofibromin is ubiquitously expressed, but expression levels may vary depending on the tissue type and developmental stage of the organism. Expression may be at its highest level in adult neurons, Schwann cells, astrocytes, leukocytes, and oligodendrocytes. Schwann cells (also referred to as neurolemmocytes) are the principal glia of the peripheral nervous system (PNS). Glial cells function to support neurons. The two types of Schwann cells are myelinating and nonmyelinating. Myelinating Schwann cells wrap around axons of motor and sensory neurons to form the myelin sheath. Schwann cells are involved in many aspects of peripheral nerve biology, such as, for example, the conduction of nervous impulses along axons, nerve development and regeneration, trophic support for neurons, production of the nerve extracellular matrix, modulation of neuromuscular synaptic activity, and presentation of antigens to T-lymphocytes.
NF1 is located on the long arm of chromosome 17, position q11.2, in humans. NF1 spans over 350-kb of genomic DNA and contains 57 exons in humans. NF1 has one of the highest mutation rates amongst known human genes, however, mutation detection is often difficult because of its large size and the variety of possible mutations. The NF1 locus has a high incidence of de novo mutations, meaning that the mutations are not inherited maternally or paternally. Although the mutation rate is high, there are no mutation “hot spot” regions. Mutations tend to be distributed within the gene, although exons 3, 5, and 27 are common sites for mutations. In some embodiments, mutations in the NF1 gene affect splicing.
An NF1 gene may be a mutant NF1 gene. An NF1 gene may be a wild-type NF1 gene. An NF1 gene may have a sequence that is functionally identical to a wild-type NF1 gene, for example, the sequence may be codon-optimized but still encode for the same protein as the wild-type NF1. A mutant NF1 gene may include one or more mutations relative to the wild-type NF1 gene. Mutations may include, for example, nucleotide deletions, substitutions, additions, transversions, or combinations thereof. A mutation in the NF1 gene may affect splicing of the NF1 gene. A mutation in the NF1 gene may be a functional deletion of the NF1 gene. In some embodiments, the mutation in the NF1 gene comprises an insertion or deletion in the NF1 gene that prevents protein expression from the NF1 gene. Mutations may be in one or more exons and/or introns. Mutations may include deletions of all or parts of at least one intron and/or exon. An exon of a mutant NF1 gene may be mutated or at least partially deleted from the NF1 gene. An exon of a mutant NF1 gene may be fully deleted. A mutant NF1 gene may have a portion or fragment thereof that corresponds to the corresponding sequence in the wild-type NF1 gene. In some embodiments, a disrupted NF1 gene caused by a deleted or mutated exon can be restored in NF1 patients by adding back the corresponding wild-type exon. In some embodiments, the mutation(s) in the mutant NF1 gene is present in the 5′ portion of the gene. In some embodiments, the mutation(s) in the mutant NF1 gene is present in the 3′ portion of the gene. In some embodiments, one or more exons may be added and inserted so as to restore the corresponding mutated or deleted exon(s) in NF1.
Provided herein are CRISPR/Cas-based gene editing systems (also referred to as CRISPR/Cas-based genome editing systems). The CRISPR/Cas-based gene editing system may be used to insert a donor sequence to correct a mutant gene sequence on a chromosome and result in expression of a functional protein. The CRISPR/Cas-based gene editing system may include a Cas protein or a fusion protein, and at least one gRNA, and may also be referred to as a “CRISPR-Cas system.”
“Clustered Regularly Interspaced Short Palindromic Repeats” and “CRISPRs”, as used interchangeably herein, refers to loci containing multiple short direct repeats that are found in the genomes of approximately 40% of sequenced bacteria and 90% of sequenced archaea. The CRISPR system is a microbial nuclease system involved in defense against invading phages and plasmids that provides a form of acquired immunity. The CRISPR loci in microbial hosts contain a combination of CRISPR-associated (Cas) genes as well as non-coding RNA elements capable of programming the specificity of the CRISPR-mediated nucleic acid cleavage. Short segments of foreign DNA, called spacers, are incorporated into the genome between CRISPR repeats, and serve as a “memory” of past exposures. Cas proteins include, for example, Cas12a, Cas9, and Cascade proteins. Cas12a may also be referred to as “Cpf1.” Cas12a causes a staggered cut in double stranded DNA, while Cas9 produces a blunt cut. In some embodiments, the Cas protein comprises Cas12a. In some embodiments, the Cas protein comprises Cas9. Cas9 forms a complex with the 3′ end of the sgRNA (which may be referred interchangeably herein as “gRNA”), and the protein-RNA pair recognizes its genomic target by complementary base pairing between the 5′ end of the gRNA sequence and a predefined 20 bp DNA sequence, known as the protospacer. This complex is directed to homologous loci of pathogen DNA via regions encoded within the crRNA, i.e., the protospacers, and protospacer-adjacent motifs (PAMs) within the pathogen genome. The non-coding CRISPR array is transcribed and cleaved within direct repeats into short crRNAs containing individual spacer sequences, which direct Cas nucleases to the target site (protospacer). By simply exchanging the 20 bp recognition sequence of the expressed gRNA, the Cas9 nuclease can be directed to new genomic targets. CRISPR spacers are used to recognize and silence exogenous genetic elements in a manner analogous to RNAi in eukaryotic organisms.
Three classes of CRISPR systems (Types I, II, and III effector systems) are known. The Type II effector system carries out targeted DNA double-strand break in four sequential steps, using a single effector enzyme, Cas9, to cleave dsDNA. Compared to the Type I and Type III effector systems, which require multiple distinct effectors acting as a complex, the Type II effector system may function in alternative contexts such as eukaryotic cells. The Type II effector system consists of a long pre-crRNA, which is transcribed from the spacer-containing CRISPR locus, the Cas9 protein, and a tracrRNA, which is involved in pre-crRNA processing. The tracrRNAs hybridize to the repeat regions separating the spacers of the pre-crRNA, thus initiating dsRNA cleavage by endogenous RNase III. This cleavage is followed by a second cleavage event within each spacer by Cas9, producing mature crRNAs that remain associated with the tracrRNA and Cas9, forming a Cas9:crRNA-tracrRNA complex. Cas12a systems include crRNA for successful targeting, whereas Cas9 systems include both crRNA and tracrRNA.
The Cas9:crRNA-tracrRNA complex unwinds the DNA duplex and searches for sequences matching the crRNA to cleave. Target recognition occurs upon detection of complementarity between a “protospacer” sequence in the target DNA and the remaining spacer sequence in the crRNA. Cas9 mediates cleavage of target DNA if a correct protospacer-adjacent motif (PAM) is also present at the 3′ end of the protospacer. For protospacer targeting, the sequence must be immediately followed by the protospacer-adjacent motif (PAM), a short sequence recognized by the Cas9 nuclease that is required for DNA cleavage. Different Cas and Cas Type II systems have differing PAM requirements. For example, Cas12a may function with PAM sequences rich in thymine “T.”
An engineered form of the Type II effector system of S. pyogenes was shown to function in human cells for genome engineering. In this system, the Cas9 protein was directed to genomic target sites by a synthetically reconstituted “guide RNA” (“gRNA”, also used interchangeably herein as a chimeric single guide RNA (“sgRNA”)), which is a crRNA-tracrRNA fusion that obviates the need for RNase III and crRNA processing in general. Provided herein are CRISPR/Cas-based engineered systems for use in gene editing and treating genetic diseases. The CRISPR/Cas-based engineered systems can be designed to target any gene, including genes involved in, for example, a genetic disease, aging, tissue regeneration, or wound healing. The CRISPR/Cas-based gene editing system can include a Cas9 protein or a Cas9 fusion protein.
Cas9 protein is an endonuclease that cleaves nucleic acid and is encoded by the CRISPR loci and is involved in the Type II CRISPR system. The Cas9 protein can be from any bacterial or archaea species, including, but not limited to, Streptococcus pyogenes, Staphylococcus aureus (S. aureus), Acidovorax avenae, Actinobacillus pleuropneumoniae, Actinobacillus succinogenes, Actinobacillus suis, Actinomycessp., cycliphilus denitrificans, Aminomonas paucivorans, Bacillus cereus, Bacillus smithii, Bacillus thuringiensis, Bacteroides sp., Blastopirellula marina, Bradyrhizobiumsp., Brevibacillus laterosporus, Campylobacter coli, Campylobacter jejuni, Campylobacter lari, Candidatus Puniceispirillum, Clostridium cellulolyticum, Clostridium perfringens. Corynebacterium accolens, Corynebacterium diphtheria, Corynebacterium matruchotii, Dinoroseobacter shibae, Eubacterium dolichum, gamma proteobacterium, Gluconacetobacter diazotrophicus, Haemophilus parainfluenzae, Haemophilus sputorum, Helicobacter canadensis, Helicobacter cinaedi, Helicobacter mustelae, Ilyobacter polytropus, Kingella kingae, Lactobacillus crispatus, Listeria ivanovii, Listeria monocytogenes, Listeriaceae bacterium, Methylocystissp., Methylosinus trichosporium, Mobiluncus mulieris, Neisseria bacilliformis, Neisseria cinerea, Neisseria flavescens, Neisseria lactamica, Neisseriasp., Neisseria wadsworthii, Nitrosomonassp., Parvibaculum lavamentivorans, Pasteurella multocida, Phascolarctobacterium succinatutens, Ralstonia syzygii, Rhodopseudomonas palustris, Rhodovulumsp., Simonsiella muelleri, Sphingomonassp., Sporolactobacillus vineae, Staphylococcus lugdunensis, Streptococcussp., Subdoligranulumsp., Tistrella mobilis, Treponemasp., or Verminephrobacter eiseniae. In certain embodiments, the Cas9 molecule is a Streptococcus pyogenes Cas9 molecule (also referred herein as “SpCas9”). SpCas9 may comprise an amino acid sequence of SEQ ID NO: 20. In certain embodiments, the Cas9 molecule is a Staphylococcus aureus Cas9 molecule (also referred herein as “SaCas9”). SaCas9 may comprise an amino acid sequence of SEQ ID NO: 21.
A Cas9 molecule or a Cas9 fusion protein can interact with one or more gRNA molecule(s) and, in concert with the gRNA molecule(s), can localize to a site which comprises a target domain, and in certain embodiments, a PAM sequence. The Cas9 protein forms a complex with the 3′ end of a gRNA. The ability of a Cas9 molecule or a Cas9 fusion protein to recognize a PAM sequence can be determined, for example, by using a transformation assay as known in the art.
The specificity of the CRISPR-based system may depend on two factors: the target sequence and the protospacer-adjacent motif (PAM). The target sequence is located on the 5′ end of the gRNA and is designed to bond with base pairs on the host DNA at the correct DNA sequence known as the protospacer. By simply exchanging the recognition sequence of the gRNA, the Cas9 protein can be directed to new genomic targets. The PAM sequence is located on the DNA to be altered and is recognized by a Cas9 protein. PAM recognition sequences of the Cas9 protein can be species specific.
In certain embodiments, the ability of a Cas9 molecule or a Cas9 fusion protein to interact with and cleave a target nucleic acid is PAM sequence dependent. A PAM sequence is a sequence in the target nucleic acid. In certain embodiments, cleavage of the target nucleic acid occurs upstream from the PAM sequence. Cas9 molecules from different bacterial species can recognize different sequence motifs (for example, PAM sequences). A Cas9 molecule of S. pyogenes may recognize the PAM sequence of NRG (5′-NRG-3′, where R is any nucleotide residue, and in some embodiments, R is either A or G, SEQ ID NO: 1). In certain embodiments, a Cas9 molecule of S. pyogenes may naturally prefer and recognize the sequence motif NGG (SEQ ID NO: 2) and directs cleavage of a target nucleic acid sequence 1 to 10, for example, 3 to 5, bp upstream from that sequence. In some embodiments, a Cas9 molecule of S. pyogenes accepts other PAM sequences, such as NAG (SEQ ID NO: 3) in engineered systems (Hsu et al., Nature Biotechnology 2013 doi:10.1038/nbt.2647). In certain embodiments, a Cas9 molecule of S. thermophilus recognizes the sequence motif NGGNG (SEQ ID NO: 4) and/or NNAGAAW (W = A or T) (SEQ ID NO: 5) and directs cleavage of a target nucleic acid sequence 1 to 10, for example, 3 to 5, bp upstream from these sequences. In certain embodiments, a Cas9 molecule of S. mutans recognizes the sequence motif NGG (SEQ ID NO: 2) and/or NAAR (R = A or G) (SEQ ID NO: 6) and directs cleavage of a target nucleic acid sequence 1 to 10, for example, 3 to 5 bp, upstream from this sequence. In certain embodiments, a Cas9 molecule of S. aureus recognizes the sequence motif NNGRR (R = A or G) (SEQ ID NO: 7) and directs cleavage of a target nucleic acid sequence 1 to 10, for example, 3 to 5, bp upstream from that sequence. In certain embodiments, a Cas9 molecule of S. aureus recognizes the sequence motif NNGRRN (R = A or G) (SEQ ID NO: 8) and directs cleavage of a target nucleic acid sequence 1 to 10, for example, 3 to 5, bp upstream from that sequence. In certain embodiments, a Cas9 molecule of S. aureus recognizes the sequence motif NNGRRT (R = A or G) (SEQ ID NO: 9) and directs cleavage of a target nucleic acid sequence 1 to 10, for example, 3 to 5, bp upstream from that sequence. In certain embodiments, a Cas9 molecule of S. aureus recognizes the sequence motif NNGRRV (R = A or G; V = A or C or G) (SEQ ID NO: 10) and directs cleavage of a target nucleic acid sequence 1 to 10, for example, 3 to 5, bp upstream from that sequence. A Cas9 molecule derived from Neisseria meningitidis (NmCas9) normally has a native PAM of NNNNGATT (SEQ ID NO: 11), but may have activity across a variety of PAMs, including a highly degenerate NNNNGNNN PAM (SEQ ID NO: 12) (Esvelt et al. Nature Methods 2013 doi:10.1038/nmeth.2681). In the aforementioned embodiments, N can be any nucleotide residue, for example, any of A, G, C, or T. Cas9 molecules can be engineered to alter the PAM specificity of the Cas9 molecule.
In some embodiments, the Cas9 protein recognizes a PAM sequence NGG (SEQ ID NO: 2) or NGA (SEQ ID NO: 13) or NNNRRT (R = A or G) (SEQ ID NO: 14) or ATTCCT (SEQ ID NO: 15) or NGAN (SEQ ID NO: 16) or NGNG (SEQ ID NO: 17). In some embodiments, the Cas9 protein is a Cas9 protein of S. aureus and recognizes the sequence motif NNGRR (R = A or G) (SEQ ID NO: 7), NNGRRN (R = A or G) (SEQ ID NO: 8), NNGRRT (R = A or G) (SEQ ID NO: 9), or NNGRRV (R = A or G; V = A or C or G) (SEQ ID NO: 10). In the aforementioned embodiments, N can be any nucleotide residue, for example, any of A, G, C, or T.
Additionally or alternatively, a nucleic acid encoding a Cas9 molecule or Cas9 polypeptide may comprise a nuclear localization sequence (NLS). Nuclear localization sequences are known in the art, for example, SV40 NLS (Pro-Lys-Lys-Lys-Arg-Lys-Val; SEQ ID NO: 35).
In some embodiments, the Cas9 protein is a VQR variant. The VQR variant of Cas9 is a mutant with a different PAM recognition, as detailed in Kleinstiver, et al. (Nature 2015, 523, 481-485, incorporated herein by reference).
A polynucleotide encoding a Cas9 molecule can be a synthetic polynucleotide. For example, the synthetic polynucleotide can be chemically modified. The synthetic polynucleotide can be codon optimized, for example, at least one non-common codon or less-common codon has been replaced by a common codon. For example, the synthetic polynucleotide can direct the synthesis of an optimized messenger mRNA, for example, optimized for expression in a mammalian expression system, as described herein. An exemplary codon optimized nucleic acid sequence encoding a Cas9 molecule of S. pyogenes is set forth in SEQ ID NO: 26. Exemplary codon optimized nucleic acid sequences encoding a Cas9 molecule of S. aureus, and optionally containing nuclear localization sequences (NLSs), are set forth in SEQ ID NOs: 27-33. Another exemplary codon optimized nucleic acid sequence encoding a Cas9 molecule of S. aureus comprises the nucleotides 1293-4451 of SEQ ID NO: 34.
The CRISPR/Cas-based gene editing system includes at least one gRNA molecule. For example, the CRISPR/Cas-based gene editing system may include two gRNA molecules. The at least one gRNA molecule can recognize and bind a target region. The gRNA is the part of the CRISPR-Cas system that provides DNA targeting specificity to the CRISPR/Cas-based gene editing system. The gRNA is a fusion of two noncoding RNAs: a crRNA and a tracrRNA. gRNA mimics the naturally occurring crRNA:tracrRNA duplex involved in the Type II Effector system. This duplex, which may include, for example, a 42-nucleotide crRNA and a 75-nucleotide tracrRNA, acts as a guide for the Cas9 to bind, and in some cases, cleave the target nucleic acid. The gRNA may target any desired DNA sequence by exchanging the sequence encoding a 20 bp protospacer which confers targeting specificity through complementary base pairing with the desired DNA target. The “target region” or “target sequence” or “protospacer” refers to the region of the target gene to which the CRISPR/Cas-based gene editing system targets and binds. The portion of the gRNA that targets the target sequence in the genome may be referred to as the “targeting sequence” or “targeting portion” or “targeting domain.” “Protospacer” or “gRNA spacer” may refer to the region of the target gene to which the CRISPR/Cas-based gene editing system targets and binds; “protospacer” or “gRNA spacer” may also refer to the portion of the gRNA that is complementary to the targeted sequence in the genome. The gRNA may include a gRNA scaffold. A gRNA scaffold facilitates Cas9 binding to the gRNA and may facilitate endonuclease activity. The gRNA scaffold is a polynucleotide sequence that follows the portion of the gRNA corresponding to sequence that the gRNA targets. Together, the gRNA targeting portion and gRNA scaffold form one polynucleotide. The constant region of the gRNA may include the sequence of SEQ ID NO: 19 (RNA), which is encoded by a sequence comprising SEQ ID NO: 18 (DNA). The CRISPR/Cas-based gene editing system may include at least one gRNA, wherein the gRNAs target different DNA sequences. The target DNA sequences may be overlapping. The gRNA may comprise at its 5′ end the targeting domain that is sufficiently complementary to the target region to be able to hybridize to, for example, about 10 to about 20 nucleotides of the target region of the target gene, when it is followed by an appropriate Protospacer Adjacent Motif (PAM). The target region or protospacer is followed by a PAM sequence at the 3′ end of the protospacer in the genome. Different Type II systems have differing PAM requirements, as detailed above.
The targeting domain of the gRNA does not need to be perfectly complementary to the target region of the target DNA. In some embodiments, the targeting domain of the gRNA is at least 80%, 85%, 90%, 95%, 96%, 97%, 98%, or at least 99% complementary to (or has 1, 2 or 3 mismatches compared to) the target region over a length of, such as, 10, 11, 12, 13, 14, 15, 16, 17, 18, 19, or 20 nucleotides. For example, the DNA-targeting domain of the gRNA may be at least 80% complementary over at least 18 nucleotides of the target region. The target region may be on either strand of the target DNA.
The gRNA may target a region within the NF1 gene. The gRNA may target a fragment or portion of a wild-type NF1 gene. The gRNA may target a fragment or portion of a mutant NF1 gene. The gRNA may target a sequence in a middle region of the NF1 gene. The middle region of the NF1 gene may include the middle 5%, 10%, 15%, 20%, 25%, 30%, 33%, or 35% of the nucleotide sequence of the gene. For example, the gRNA may target a sequence within an intronic region between exon 30 and exon 31 of the NF1 gene. As further detailed below, the gRNA may target a sequence in a vector. The gRNA may bind and target and/or hybridize to a polynucleotide sequence comprising at least one of SEQ ID NOs: 49-59, or a complement thereof, or a variant thereof, or a truncation thereof, as shown in TABLE 1. The gRNA may be encoded by a polynucleotide sequence comprising at least one of SEQ ID NOs: 60-70, or a complement thereof, or a variant thereof, or a truncation thereof (TABLE 2). The gRNA may comprise a polynucleotide sequence selected from SEQ ID NOs: 71-81, or a complement thereof, or a variant thereof, or a truncation thereof (TABLE 2). The gRNA may bind and target and/or hybridize to, and/or be encoded by, and/or comprise, a polynucleotide sequence comprising at least one of SEQ ID NOs: 49-81, or a complement thereof, or a variant thereof, or a truncation thereof. A truncation may be 1, 2, 3, 4, 5, 6, 7, 8, or 9 nucleotides shorter than the reference sequence.
As described above, the gRNA molecule comprises a targeting domain (also referred to as targeted or targeting sequence), which is a polynucleotide sequence complementary to the target DNA sequence. The gRNA may comprise a “G” at the 5′ end of the targeting domain or complementary polynucleotide sequence. The CRISPR/Cas-based gene editing system may use gRNAs of varying sequences and lengths. The targeting domain of a gRNA molecule may comprise at least a 10 base pair, at least a 11 base pair, at least a 12 base pair, at least a 13 base pair, at least a 14 base pair, at least a 15 base pair, at least a 16 base pair, at least a 17 base pair, at least a 18 base pair, at least a 19 base pair, at least a 20 base pair, at least a 21 base pair, at least a 22 base pair, at least a 23 base pair, at least a 24 base pair, at least a 25 base pair, at least a 30 base pair, or at least a 35 base pair complementary polynucleotide sequence of the target DNA sequence followed by a PAM sequence. In certain embodiments, the targeting domain of a gRNA molecule has 19-25 nucleotides in length. In certain embodiments, the targeting domain of a gRNA molecule is 20 nucleotides in length. In certain embodiments, the targeting domain of a gRNA molecule is 21 nucleotides in length. In certain embodiments, the targeting domain of a gRNA molecule is 22 nucleotides in length. In certain embodiments, the targeting domain of a gRNA molecule is 23 nucleotides in length.
The number of gRNA molecules that may be included in the CRISPR/Cas-based gene editing system can be at least 1 gRNA, at least 2 different gRNAs, at least 3 different gRNAs, at least 4 different gRNAs, at least 5 different gRNAs, at least 6 different gRNAs, at least 7 different gRNAs, at least 8 different gRNAs, at least 9 different gRNAs, at least 10 different gRNAs, at least 11 different gRNAs, at least 12 different gRNAs, at least 13 different gRNAs, at least 14 different gRNAs, at least 15 different gRNAs, at least 16 different gRNAs, at least 17 different gRNAs, at least 18 different gRNAs, at least 18 different gRNAs, at least 20 different gRNAs, at least 25 different gRNAs, at least 30 different gRNAs, at least 35 different gRNAs, at least 40 different gRNAs, at least 45 different gRNAs, or at least 50 different gRNAs. The number of gRNA molecules that may be included in the CRISPR/Cas-based gene editing system can be less than 50 different gRNAs, less than 45 different gRNAs, less than 40 different gRNAs, less than 35 different gRNAs, less than 30 different gRNAs, less than 25 different gRNAs, less than 20 different gRNAs, less than 19 different gRNAs, less than 18 different gRNAs, less than 17 different gRNAs, less than 16 different gRNAs, less than 15 different gRNAs, less than 14 different gRNAs, less than 13 different gRNAs, less than 12 different gRNAs, less than 11 different gRNAs, less than 10 different gRNAs, less than 9 different gRNAs, less than 8 different gRNAs, less than 7 different gRNAs, less than 6 different gRNAs, less than 5 different gRNAs, less than 4 different gRNAs, less than 3 different gRNAs, or less than 2 different gRNAs. The number of gRNAs that may be included in the CRISPR/Cas-based gene editing system can be between at least 1 gRNA to at least 50 different gRNAs, at least 1 gRNA to at least 45 different gRNAs, at least 1 gRNA to at least 40 different gRNAs, at least 1 gRNA to at least 35 different gRNAs, at least 1 gRNA to at least 30 different gRNAs, at least 1 gRNA to at least 25 different gRNAs, at least 1 gRNA to at least 20 different gRNAs, at least 1 gRNA to at least 16 different gRNAs, at least 1 gRNA to at least 12 different gRNAs, at least 1 gRNA to at least 8 different gRNAs, at least 1 gRNA to at least 4 different gRNAs, at least 4 gRNAs to at least 50 different gRNAs, at least 4 different gRNAs to at least 45 different gRNAs, at least 4 different gRNAs to at least 40 different gRNAs, at least 4 different gRNAs to at least 35 different gRNAs, at least 4 different gRNAs to at least 30 different gRNAs, at least 4 different gRNAs to at least 25 different gRNAs, at least 4 different gRNAs to at least 20 different gRNAs, at least 4 different gRNAs to at least 16 different gRNAs, at least 4 different gRNAs to at least 12 different gRNAs, at least 4 different gRNAs to at least 8 different gRNAs, at least 8 different gRNAs to at least 50 different gRNAs, at least 8 different gRNAs to at least 45 different gRNAs, at least 8 different gRNAs to at least 40 different gRNAs, at least 8 different gRNAs to at least 35 different gRNAs, 8 different gRNAs to at least 30 different gRNAs, at least 8 different gRNAs to at least 25 different gRNAs, 8 different gRNAs to at least 20 different gRNAs, at least 8 different gRNAs to at least 16 different gRNAs, or 8 different gRNAs to at least 12 different gRNAs.
The CRISPR/Cas-based gene editing system may include at least one donor sequence. A donor sequence comprises a polynucleotide sequence to be inserted into a genome. A donor sequence may comprise a wild-type sequence of a gene. A donor sequence may comprise the wild-type NF1 gene. A donor sequence may comprise a fragment or portion of the wild-type NF1 gene. The fragment or portion of the NF1 gene may be, for example, about 50% of the full nucleotide sequence of the gene. The fragment or portion of the NF1 gene may be at least about 30%, at least about 35%, at least about 40%, at least about 45%, or at least about 50% of the full nucleotide sequence of the gene. The fragment or portion of the NF1 gene may be less than about 70%, less than about 65%, less than about 60%, less than about 55%, or less than about 50% of the full nucleotide sequence of the gene. The fragment or portion of the NF1 gene may include about 20-80%, about 30-70%, about 40-60%, or about 45-55% of the full nucleotide sequence of the gene. The donor sequence may include a 5′ portion or fragment of the wild-type NF1 gene. The 5′ portion or fragment of the NF1 gene may include the 5′ end of the NF1 gene including about 20-80%, about 30-70%, about 40-60%, or about 45-55% of the full nucleotide sequence of the gene. The donor sequence may include the 5′ end of the wild-type NF1 gene including about 20-80%, about 30-70%, about 40-60%, or about 45-55% of the full nucleotide sequence of the gene. The donor sequence may include a 3′ portion or fragment of the wild-type NF1 gene. The 3′ portion or fragment of the NF1 gene may include the 3′ end of the NF1 gene including about 20-80%, about 30-70%, about 40-60%, or about 45-55% of the full nucleotide sequence of the gene. The donor sequence may include the 3′ end of the wild-type NF1 gene including about 20-80%, about 30-70%, about 40-60%, or about 45-55% of the full nucleotide sequence of the gene.
A donor sequence may comprise multiple exons of the wild-type NF1 gene. In some embodiments, the donor sequence comprises one or more exons selected from exon 1, exon 2, exon 3, exon 4, exon 5, exon 6, exon 7, exon 8, exon 9, exon 10, exon 11, exon 12, exon 13, exon 14, exon 15, exon 16, exon 17, exon 18, exon 19, exon 20, exon 21, exon 22, exon 23, exon 24, exon 25, exon 26, exon 27, exon 28, exon 29, exon 30, exon 31, exon 32, exon 33, exon 34, exon 35, exon 36, exon 37, exon 38, exon 39, exon 40, exon 41, exon 42, exon 43, exon 44, exon 45, exon 46, exon 47, exon 48, exon 49, exon 50, exon 51, exon 52, exon 53, exon 54, exon 55, exon 56, and exon 57 of the wild-type NF1 gene or a functional equivalent thereof. In some embodiments, the donor sequence comprises one or more contiguous exons of the wild-type NF1 gene or a functional equivalent thereof. In some embodiments, the donor sequence comprises exons 1-30 of the wild-type NF1 gene.
The donor sequence may comprise a polynucleotide sequence of SEQ ID NO: 82.
The gRNA and donor sequence may be present in a variety of molar ratios. The molar ratio between the gRNA and donor sequence may be 1:1, or 1:15, or from 5:1 to 1:10, or from 1:1 to 1:5. The molar ratio between the gRNA and donor sequence may be at least 1:1, at least 1:2, at least 1:3, at least 1:4, at least 1:5, at least 1:6, at least 1:7, at least 1:8, at least 1:9, at least 1:10, at least 1:15, or at least 1:20. The molar ratio between the gRNA and donor sequence may be less than 20:1, less than 15:1, less than 10:1, less than 9:1, less than 8:1, less than 7:1, less than 6:1, less than 5:1, less than 4:1, less than 3:1, less than 2:1, or less than 1:1.
The CRISPR/Cas-based gene editing system may be used to introduce site-specific double strand breaks at targeted genomic loci, such as a location within the NF1 gene. Site-specific double-strand breaks are created when the CRISPR/Cas-based gene editing system binds to a target DNA sequences, thereby permitting cleavage of the target DNA. This DNA cleavage may stimulate the natural DNA-repair machinery, leading to one of two possible repair pathways: homology-directed repair (HDR) or the non-homologous end joining (NHEJ) pathway.
Restoration of protein expression from a gene may involve homology-directed repair (HDR). A donor template may be administered to a cell. The donor template may include a nucleotide sequence encoding a full-functional protein or a partially functional protein. In such embodiments, the donor template may include fully functional gene construct for restoring a mutant gene, or a fragment of the gene that after homology-directed repair, leads to restoration of the mutant gene. In other embodiments, the donor template may include a nucleotide sequence encoding a mutated version of an inhibitory regulatory element of a gene. Mutations may include, for example, nucleotide substitutions, insertions, deletions, or a combination thereof. In such embodiments, introduced mutation(s) into the inhibitory regulatory element of the gene may reduce the transcription of or binding to the inhibitory regulatory element.
Restoration of protein expression from gene may be through template-free NHEJ-mediated DNA repair. In certain embodiments, NHEJ is a nuclease mediated NHEJ, which in certain embodiments, refers to NHEJ that is initiated a Cas9 molecule that cuts double stranded DNA. The method comprises administering a presently disclosed CRISPR/Cas-based gene editing system or a composition comprising thereof to a subject for gene editing.
Nuclease mediated NHEJ may correct a mutated target gene and offer several potential advantages over the HDR pathway. For example, NHEJ does not require a donor template, which may cause nonspecific insertional mutagenesis. In contrast to HDR, NHEJ operates efficiently in all stages of the cell cycle and therefore may be effectively exploited in both cycling and post-mitotic cells, such as muscle fibers. This provides a robust, permanent gene restoration alternative to oligonucleotide-based exon skipping or pharmacologic forced read-through of stop codons and could theoretically require as few as one drug treatment.
The CRISPR/Cas-based gene editing system may be encoded by or comprised within one or more genetic constructs. The CRISPR/Cas-based gene editing system may comprise one or more genetic constructs. The genetic construct, such as a plasmid or expression vector, may comprise a nucleic acid that encodes the CRISPR/Cas-based gene editing system and/or at least one gRNA and/or a donor sequence.
In some embodiments, the CRISPR/Cas-based gene editing system includes two vectors: a first vector and a second vector. The first vector may encode a Cas protein or a fusion protein, and at least one gRNA. The polynucleotide sequence encoding the gRNA and the polynucleotide sequence encoding the Cas protein or the fusion protein may be operably linked. The second vector may encode a donor sequence.
In some embodiments, the polynucleotide sequence encoding the donor sequence further comprises a stop codon. The stop codon may be 5′ or 3′ to the donor sequence. The stop codon may be upstream or downstream of the donor sequence. The stop codon and the donor sequence may be in the same reading frame.
The vector may further encode a promoter. The first vector may encode a promoter 5′ to or upstream of the polynucleotide encoding the Cas protein or the fusion protein. The first vector may encode a promoter 5′ to or upstream of the polynucleotide encoding the at least one gRNA. The second vector may encode a promoter 5′ to or upstream of the donor sequence. The promoters may be the same or different.
In some embodiments, the mutant NF1 gene comprises a mutation in the 5′ portion of the mutant NF1 gene, and the polynucleotide sequence encoding the donor sequence further comprises a stop codon that is 5′ to or upstream of the donor sequence. As detailed above, the 5′ portion or fragment of the NF1 gene may include the 3′ end of the NF1 gene including about 20-80%, about 30-70%, about 40-60%, or about 45-55% of the full nucleotide sequence of the gene. The polynucleotide sequence may further include a promoter in between the stop codon and the donor sequence. The stop codon, the promoter, and the donor sequence may be flanked on both ends (the 5′ and 3′ ends) with a sequence the gRNA targets. In such embodiments, the gRNA targets a sequence upstream of the stop codon that is 5′ to or upstream of the donor sequence in the second vector, and also targets a sequence 3′ to or downstream of the donor sequence in the second vector. In some embodiments, upon integration of the donor sequence into the chromosome, the stop codon, the donor sequence, and the 3′ portion of the mutant NF1 gene are in the same reading frame.
In some embodiments, the mutant NF1 gene comprises a mutation in the 3′ portion of the mutant NF1 gene, and the polynucleotide sequence encoding the donor sequence further comprises a stop codon that is 3′ to or downstream of the donor sequence. As detailed above, the 3′ portion or fragment of the NF1 gene may include the 3′ end of the NF1 gene including about 20-80%, about 30-70%, about 40-60%, or about 45-55% of the full nucleotide sequence of the gene. The stop codon and the donor sequence may be flanked on both ends (the 5′ and 3′ ends) with a sequence the gRNA targets. In such embodiments, the gRNA targets a sequence 5′ to or upstream of the donor sequence in the second vector, and also targets a sequence 3′ to or downstream of the stop codon that is 5′ to or upstream of the donor sequence in the second vector. In some embodiments, upon integration of the donor sequence into the chromosome, the 5′ portion of the mutant NF1 gene, the donor sequence, and the stop codon are in the same reading frame. In some embodiments, upon integration of the donor sequence into the chromosome, the 5′ portion of the mutant NF1 gene, the donor sequence, and the stop codon are in the same reading frame, such that the donor sequence and 5′ portion of the chromosomal NF1 gene would be transcribed together and rely on the endogenous promoter.
The promoters may be a constitutive promoter, an inducible promoter, a repressible promoter, or a regulatable promoter. The promoter may be a ubiquitous promoter. The promoter may be a tissue-specific promoter. The tissue specific promoter may be a muscle specific promoter. The tissue specific promoter may be a skin specific promoter. The CRISPR/Cas-based gene editing system may be under the light-inducible or chemically inducible control to enable the dynamic control of gene/genome editing in space and time. The promoter operably linked to the CRISPR/Cas-based gene editing system coding sequence may be a promoter from simian virus 40 (SV40), a mouse mammary tumor virus (MMTV) promoter, a human immunodeficiency virus (HIV) promoter such as the bovine immunodeficiency virus (BlV) long terminal repeat (LTR) promoter, a Moloney virus promoter, an avian leukosis virus (ALV) promoter, a cytomegalovirus (CMV) promoter such as the CMV immediate early promoter, Epstein Barr virus (EBV) promoter, or a Rous sarcoma virus (RSV) promoter. The promoter may also be a promoter from a human gene such as human ubiquitin C (hUbC), human actin, human myosin, human hemoglobin, human muscle creatine, or human metalothionein. Examples of a tissue specific promoter, such as a muscle or skin specific promoter, natural or synthetic, are described in U.S. Pat. Application Publication No. US20040175727, the contents of which are incorporated herein in its entirety. The promoter may be a CK8 promoter, a Spc512 promoter, a MHCK7 promoter, for example. In some embodiments, the vector may also comprise an additional promoter that is operably linked to the CRISPR/Cas-based gene editing system coding sequence.
In certain embodiments, a genetic construct encodes one gRNA molecule, i.e., a first gRNA molecule, and optionally a Cas9 molecule or fusion protein. In some embodiments, a genetic construct encodes two gRNA molecules, i.e., a first gRNA molecule and a second gRNA molecule, and optionally a Cas9 molecule or fusion protein. In some embodiments, a first genetic construct encodes one gRNA molecule, i.e., a first gRNA molecule, and optionally a Cas9 molecule or fusion protein, and a second genetic construct encodes one gRNA molecule, i.e., a second gRNA molecule, and optionally a Cas9 molecule or fusion protein. In some embodiments, a first genetic construct encodes one gRNA molecule and one donor sequence, and a second genetic construct encodes a Cas9 molecule or fusion protein. In some embodiments, a first genetic construct encodes one gRNA molecule and a Cas9 molecule or fusion protein, and a second genetic construct encodes one donor sequence.
Genetic constructs may include polynucleotides such as vectors and plasmids. The genetic construct may be a linear minichromosome including centromere, telomeres, or plasmids or cosmids. The vector may be an expression vectors or system to produce protein by routine techniques and readily available starting materials including Sambrook et al., Molecular Cloning and Laboratory Manual, Second Ed., Cold Spring Harbor (1989), which is incorporated fully by reference. The construct may be recombinant. The genetic construct may be part of a genome of a recombinant viral vector, including recombinant lentivirus, recombinant adenovirus, and recombinant adenovirus associated virus. The genetic construct may comprise regulatory elements for gene expression of the coding sequences of the nucleic acid. The regulatory elements may be a promoter, an enhancer, an initiation codon, a stop codon, or a polyadenylation signal.
The genetic construct may comprise heterologous nucleic acid encoding the CRISPR/Cas-based gene editing system and may further comprise an initiation codon, which may be upstream of the CRISPR/Cas-based gene editing system coding sequence, and another stop codon, which may be downstream of the CRISPR/Cas-based gene editing system coding sequence. The genetic construct may include more than one stop codon, which may be downstream of the CRISPR/Cas-based gene editing system coding sequence. In some embodiments, the genetic construct includes 1, 2, 3, 4, or 5 stop codons. In some embodiments, the genetic construct includes 1, 2, 3, 4, or 5 stop codons downstream of the sequence encoding the donor sequence. A stop codon may be in-frame with a coding sequence in the CRISPR/Cas-based gene editing system. For example, one or more stop codons may be in-frame with the donor sequence. The genetic construct may include one or more stop codons that are out of frame of a coding sequence in the CRISPR/Cas-based gene editing system. For example, one stop codon may be in-frame with the donor sequence, and two other stop codons may be included that are in the other two possible reading frames. A genetic construct may include a stop codon for all three potential reading frames. The initiation and termination codon may be in frame with the CRISPR/Cas-based gene editing system coding sequence.
The genetic construct may also comprise a polyadenylation signal, which may be downstream of the CRISPR/Cas-based gene editing system. The polyadenylation signal may be a SV40 polyadenylation signal, LTR polyadenylation signal, bovine growth hormone (bGH) polyadenylation signal, human growth hormone (hGH) polyadenylation signal, or human β-globin polyadenylation signal. The SV40 polyadenylation signal may be a polyadenylation signal from a pCEP4 vector (Invitrogen, San Diego, CA).
Coding sequences in the genetic construct may be optimized for stability and high levels of expression. In some instances, codons are selected to reduce secondary structure formation of the RNA such as that formed due to intramolecular bonding.
The genetic construct may also comprise an enhancer upstream of the CRISPR/Cas-based gene editing system or gRNAs. The enhancer may be necessary for DNA expression. The enhancer may be human actin, human myosin, human hemoglobin, human muscle creatine or a viral enhancer such as one from CMV, HA, RSV, or EBV. Polynucleotide function enhancers are described in U.S. Pat. Nos. 5,593,972, 5,962,428, and WO94/016737, the contents of each are fully incorporated by reference. The genetic construct may also comprise a mammalian origin of replication in order to maintain the vector extrachromosomally and produce multiple copies of the vector in a cell. The genetic construct may also comprise a regulatory sequence, which may be well suited for gene expression in a mammalian or human cell into which the vector is administered. The genetic construct may also comprise a reporter gene, such as green fluorescent protein (“GFP”) and/or a selectable marker, such as hygromycin (“Hygro”).
The genetic construct may be useful for transfecting cells with nucleic acid encoding the CRISPR/Cas-based gene editing system, which the transformed host cell is cultured and maintained under conditions wherein expression of the CRISPR/Cas-based gene editing system takes place. The genetic construct may be transformed or transduced into a cell. The genetic construct may be formulated into any suitable type of delivery vehicle including, for example, a viral vector, lentiviral expression, mRNA electroporation, and lipid-mediated transfection for delivery into a cell. The genetic construct may be part of the genetic material in attenuated live microorganisms or recombinant microbial vectors which live in cells. The genetic construct may be present in the cell as a functioning extrachromosomal molecule.
Further provided herein is a cell transformed or transduced with a system or component thereof as detailed herein. Suitable cell types are detailed herein. In some embodiments, the cell is a stem cell. The stem cell may be a human stem cell. In some embodiments, the cell is an embryonic stem cell. The stem cell may be a human pluripotent stem cell (iPSCs). Further provided are stem cell-derived neurons, such as neurons derived from iPSCs transformed or transduced with a DNA targeting system or component thereof as detailed herein.
A genetic construct may be a viral vector. Further provided herein is a viral delivery system. Viral delivery systems may include, for example, lentivirus, retrovirus, adenovirus, mRNA electroporation, or nanoparticles. In some embodiments, the vector is a modified lentiviral vector. In some embodiments, the viral vector is an adeno-associated virus (AAV) vector. The AAV vector is a small virus belonging to the genus Dependovirus of the Parvoviridae family that infects humans and some other primate species.
AAV vectors may be used to deliver CRISPR/Cas-based gene editing systems using various construct configurations. For example, AAV vectors may deliver Cas9 or fusion protein and gRNA expression cassettes on separate vectors or on the same vector. Alternatively, if the small Cas9 proteins or fusion proteins, derived from species such as Staphylococcus aureus or Neisseria meningitidis, are used then both the Cas9 and up to two gRNA expression cassettes may be combined in a single AAV vector. In some embodiments, the AAV vector has a 4.7 kb packaging limit.
In some embodiments, the AAV vector is a modified AAV vector. The modified AAV vector may have enhanced cardiac and/or skeletal muscle tissue tropism. The modified AAV vector may be capable of delivering and expressing the CRISPR/Cas-based gene editing system in the cell of a mammal. For example, the modified AAV vector may be an AAV-SASTG vector (Piacentino et al. Human Gene Therapy 2012, 23, 635-646). The modified AAV vector may be based on one or more of several capsid types, including AAV1, AAV2, AAV5, AAV6, AAV8, and AAV9. The modified AAV vector may be based on AAV2 pseudotype with alternative muscle-tropic AAV capsids, such as AAV2/1, AAV2/6, AAV2/7, AAV2/8, AAV2/9, AAV2.5, and AAV/SASTG vectors that efficiently transduce skeletal muscle or cardiac muscle by systemic and local delivery (Seto et al. Current Gene Therapy 2012, 12, 139-151). The modified AAV vector may be AAV2i8G9 (Shen et al. J. Biol. Chem. 2013, 288, 28814-28823).
The genetic construct may comprise a polynucleotide sequence selected from SEQ ID NOs: 83-86, 87-90, 91-102, a complement thereof, or a fragment thereof.
Further provided herein are pharmaceutical compositions comprising the above-described genetic constructs or gene editing systems. In some embodiments, the pharmaceutical composition may comprise about 1 ng to about 10 mg of DNA encoding the CRISPR/Cas-based gene editing system. The systems or genetic constructs as detailed herein, or at least one component thereof, may be formulated into pharmaceutical compositions in accordance with standard techniques well known to those skilled in the pharmaceutical art. The pharmaceutical compositions can be formulated according to the mode of administration to be used. In cases where pharmaceutical compositions are injectable pharmaceutical compositions, they are sterile, pyrogen free, and particulate free. An isotonic formulation is preferably used. Generally, additives for isotonicity may include sodium chloride, dextrose, mannitol, sorbitol and lactose. In some cases, isotonic solutions such as phosphate buffered saline are preferred. Stabilizers include gelatin and albumin. In some embodiments, a vasoconstriction agent is added to the formulation.
The composition may further comprise a pharmaceutically acceptable excipient. The pharmaceutically acceptable excipient may be functional molecules as vehicles, adjuvants, carriers, or diluents. The term “pharmaceutically acceptable carrier,” may be a non-toxic, inert solid, semi-solid or liquid filler, diluent, encapsulating material or formulation auxiliary of any type. Pharmaceutically acceptable carriers include, for example, diluents, lubricants, binders, disintegrants, colorants, flavors, sweeteners, antioxidants, preservatives, glidants, solvents, suspending agents, wetting agents, surfactants, emollients, propellants, humectants, powders, pH adjusting agents, and combinations thereof. The pharmaceutically acceptable excipient may be a transfection facilitating agent, which may include surface active agents, such as immune-stimulating complexes (ISCOMS), Freunds incomplete adjuvant, LPS analog including monophosphoryl lipid A, muramyl peptides, quinone analogs, vesicles such as squalene and squalene, hyaluronic acid, lipids, liposomes, calcium ions, viral proteins, polyanions, polycations, or nanoparticles, or other known transfection facilitating agents. The transfection facilitating agent may be a polyanion, polycation, including poly-L-glutamate (LGS), or lipid. The transfection facilitating agent may be poly-L-glutamate, and more preferably, the poly-L-glutamate may be present in the composition for gene editing in skeletal muscle or cardiac muscle at a concentration less than 6 mg/mL.
The systems or genetic constructs as detailed herein, or at least one component thereof, may be administered or delivered to a cell. Methods of introducing a nucleic acid into a host cell are known in the art, and any known method can be used to introduce a nucleic acid (e.g., an expression construct) into a cell. Suitable methods include, for example, viral or bacteriophage infection, transfection, conjugation, protoplast fusion, polycation or lipid:nucleic acid conjugates, lipofection, electroporation, nucleofection, immunoliposomes, calcium phosphate precipitation, polyethyleneimine (PEI)-mediated transfection, DEAE-dextran mediated transfection, liposome-mediated transfection, particle gun technology, calcium phosphate precipitation, direct micro injection, nanoparticle-mediated nucleic acid delivery, and the like. In some embodiments, the composition may be delivered by mRNA delivery and ribonucleoprotein (RNP) complex delivery. The system, genetic construct, or composition comprising the same, may be electroporated using BioRad Gene Pulser Xcell or Amaxa Nucleofector IIb devices or other electroporation device. Several different buffers may be used, including BioRad electroporation solution, Sigma phosphate-buffered saline product #D8537 (PBS), Invitrogen OptiMEM I (OM), or Amaxa Nucleofector solution V (N.V.). Transfections may include a transfection reagent, such as Lipofectamine 2000.
The systems or genetic constructs as detailed herein, or at least one component thereof, or the pharmaceutical compositions comprising the same, may be administered to a subject. Such compositions can be administered in dosages and by techniques well known to those skilled in the medical arts taking into consideration such factors as the age, sex, weight, and condition of the particular subject, and the route of administration. The presently disclosed systems, or at least one component thereof, genetic constructs, or compositions comprising the same, may be administered to a subject by different routes including orally, parenterally, sublingually, transdermally, rectally, transmucosally, topically, intranasal, intravaginal, via inhalation, via buccal administration, intrapleurally, intravenous, intraarterial, intraperitoneal, subcutaneous, intradermally, epidermally, intramuscular, intranasal, intrathecal, intracranial, and intraarticular or combinations thereof. In certain embodiments, the system, genetic construct, or composition comprising the same, is administered to a subject intramuscularly, intravenously, or a combination thereof. The systems, genetic constructs, or compositions comprising the same may be delivered to a subject by several technologies including DNA injection (also referred to as DNA vaccination) with and without in vivo electroporation, liposome mediated, nanoparticle facilitated, recombinant vectors such as recombinant lentivirus, recombinant adenovirus, and recombinant adenovirus associated virus. The composition may be injected into the brain or other component of the central nervous system. The composition may be injected into the skeletal muscle or cardiac muscle. For example, the composition may be injected into the tibialis anterior muscle or tail. For veterinary use, the systems, genetic constructs, or compositions comprising the same may be administered as a suitably acceptable formulation in accordance with normal veterinary practice. The veterinarian may readily determine the dosing regimen and route of administration that is most appropriate for a particular animal. The systems, genetic constructs, or compositions comprising the same may be administered by traditional syringes, needleless injection devices, “microprojectile bombardment gone guns,” or other physical methods such as electroporation (“EP”), “hydrodynamic method”, or ultrasound. Alternatively, transient in vivo delivery of CRISPR/Cas-based systems by non-viral or non-integrating viral gene transfer, or by direct delivery of purified proteins and gRNAs containing cell-penetrating motifs may enable highly specific correction and/or restoration in situ with minimal or no risk of exogenous DNA integration.
Upon delivery of the presently disclosed systems or genetic constructs as detailed herein, or at least one component thereof, or the pharmaceutical compositions comprising the same, and thereupon the vector into the cells of the subject, the transfected cells may express the gRNA molecule(s) and the Cas9 molecule or fusion protein.
Any of the delivery methods and/or routes of administration detailed herein can be utilized with a myriad of cell types. Further provided herein is a cell transformed or transduced with a system or component thereof as detailed herein. For example, provided herein is a cell comprising an isolated polynucleotide encoding a CRISPR/Cas system as detailed herein. Suitable cell types are detailed herein. In some embodiments, the cell is an immune cell. Immune cells may include, for example, lymphocytes such as T cells and B cells and natural killer (NK) cells. In some embodiments, the cell is a T cell. T cells may be divided into cytotoxic T cells and helper T cells, which are in turn categorized as TH1 or TH2 helper T cells. Immune cells may further include innate immune cells, adaptive immune cells, tumor-primed T cells, NKT cells, IFN-y producing killer dendritic cells (IKDC), memory T cells (TCMs), and effector T cells (TEs). The cell may be a stem cell such as a human stem cell. In some embodiments, the cell is an embryonic stem cell or a hematopoietic stem cell. The stem cell may be a human induced pluripotent stem cell (iPSCs). Further provided are stem cell-derived neurons, such as neurons derived from iPSCs transformed or transduced with a DNA targeting system or component thereof as detailed herein. The cell may be a muscle cell. Cells may further include, but are not limited to, immortalized myoblast cells, dermal fibroblasts, bone marrow-derived progenitors, skeletal muscle progenitors, human skeletal myoblasts, CD 133+ cells, mesoangioblasts, cardiomyocytes, hepatocytes, chondrocytes, mesenchymal progenitor cells, hematopoietic stem cells, smooth muscle cells, and MyoD- or Pax7-transduced cells, or other myogenic progenitor cells.
Provided herein is a kit, which may be used to modify or correct a NF1 gene, or to restore NF1 function, in a cell or a subject in need thereof. The kit comprises genetic constructs or a composition comprising the same, or a component thereof, for modifying or correcting a NF1 gene, or for restoring NF1 function, as described above, and instructions for using said composition or component thereof. In some embodiments, the kit comprises at least one gRNA comprising a polynucleotide sequence of one of SEQ ID NOs: 71-81, a complement thereof, a variant thereof, a truncation thereof, or fragment thereof, and/or at least one gRNA encoded by a polynucleotide comprising a sequence of one of SEQ ID NOs: 60-70, a complement thereof, a truncation thereof, a variant thereof, or fragment thereof, and/or at least one gRNA targeting and binding and/or hybridizing to a polynucleotide comprising a sequence of one of SEQ ID NOs: 49-59, a complement thereof, a variant thereof, a truncation thereof, or fragment thereof. The kit may further include instructions for using the CRISPR/Cas-based gene editing system.
Instructions included in kits may be affixed to packaging material or may be included as a package insert. While the instructions are typically written on printed materials they are not limited to such. Any medium capable of storing such instructions and communicating them to an end user is contemplated by this disclosure. Such media include, but are not limited to, electronic storage media (e.g., magnetic discs, tapes, cartridges, chips), optical media (e.g., CD ROM), and the like. As used herein, the term “instructions” may include the address of an internet site that provides the instructions.
The genetic constructs or a composition comprising thereof for modifying or correcting a NF1 gene, or for restoring NF1 function, may include a modified AAV vector that includes a gRNA molecule(s) and a Cas9 protein or fusion protein, as described above, that specifically binds and cleaves a region of the NF1 gene. The CRISPR/Cas-based gene editing system, as described above, may be included in the kit to specifically bind and target a particular region, for example, an intronic region and/or a middle portion of the gene.
Provided herein are methods for restoring NF1 function in a cell or a subject having a mutant NF1 gene. The methods may include contacting the cell or the subject with a CRISPR/Cas-based genome editing system as detailed herein, a cell as detailed herein, or a genetic construct as detailed herein. In some embodiments, NF1 function is restored by inserting one or more wild-type exons of the NF1 gene corresponding to the mutant NF1 gene.
Further provided herein are methods for modifying or correcting a NF1 gene. The NF1 gene may be a mutant gene in a cell or in a subject. The methods may include contacting the cell or the subject with a CRISPR/Cas-based genome editing system as detailed herein, a cell as detailed herein, or a genetic construct as detailed herein. In some embodiments, NF1 function is restored by inserting one or more wild-type exons of the NF1 gene corresponding to the mutant NF1 gene.
Provided herein are methods of treating Neurofibromatosis Type I (NF1) in a cell or in a subject in need thereof. The methods may include contacting the cell or the subject with a CRISPR/Cas-based genome editing system as detailed herein, a cell as detailed herein, or a genetic construct as detailed herein. In some embodiments, NF1 function is restored by inserting one or more wild-type exons of the NF1 gene corresponding to the mutant NF1 gene.
The foregoing may be better understood by reference to the following examples, which are presented for purposes of illustration and are not intended to limit the scope of the invention. The present disclosure has multiple aspects and embodiments, illustrated by the appended non-limiting examples.
gRNAs were designed to target the middle region of the chromosomal NF1 gene, between exons 30 and 31. Shown in
Several gRNAs were designed (TABLE 1 and TABLE 2), based on targeting regions in the intronic region between exon 30 and exon 31 in chromosomal NF1 gene, low predicted off-target activity, and activity in both mice and humans. Editing efficiency was measured using the Surveyor Assay, which uses the T7 endonuclease 1 (T7E1 )(Sentmanat et al. Scientific Reports 2018, 8, 888). T7E1 is a structure-selective enzyme that detects structural deformities in heteroduplexed DNA. To detect CRISPR-Cas9-mediated gene editing, CRISPR-Cas9 reagents were transfected into cells, and the genomic DNA surrounding the target locus was amplified by PCR several days later. The PCR product was denatured and recomplexed by heating and subsequent slow cooling. If an aberrant NHEJ event occurred after CRISPR-Cas9 cleavage, a heteroduplex formed between amplicons of different lengths (for example, mutant and wild-type amplicons), leading to a DNA distortion that was recognized and cleaved by T7E1. The banding patterns of the cut products were compared between control and experimental samples to determine the frequency of mutations. Results are shown in
Donor cassettes containing the 5′ half of the NF1 cDNA were constructed for each of the top four performing gRNAs from Example 1 with the highest levels of editing activity. The gRNA and donor cassette pairs were then delivered with SaCas9 in HEK293T cells to evaluate the editing activity. Genomic DNA and RNA were harvested.
Insertion of the donor sequence was confirmed with In-Out PCR and deep sequencing. Shown in
Shown in
Shown in
Shown in
Shown in
As detailed herein, donor sequence integration has been confirmed, and transcription and correct splicing of the donor sequence into the remaining downstream portion of the gene has been shown. Donor insertion rate has been measured to be 5% of alleles.
The editing efficiency will be quantified in Schwann cells where the disease originates. The strategy will be further evaluated in human patient cell lines and in an NF1 mouse model to show that restoration of the correct NF1 sequence results in a phenotypic change and reduces Ras signaling as well as the number and size of neurofibromas.
The foregoing description of the specific aspects will so fully reveal the general nature of the invention that others can, by applying knowledge within the skill of the art, readily modify and/or adapt for various applications such specific aspects, without undue experimentation, without departing from the general concept of the present disclosure. Therefore, such adaptations and modifications are intended to be within the meaning and range of equivalents of the disclosed aspects, based on the teaching and guidance presented herein. It is to be understood that the phraseology or terminology herein is for the purpose of description and not of limitation, such that the terminology or phraseology of the present specification is to be interpreted by the skilled artisan in light of the teachings and guidance.
The breadth and scope of the present disclosure should not be limited by any of the above-described exemplary aspects, but should be defined only in accordance with the following claims and their equivalents.
All publications, patents, patent applications, and/or other documents cited in this application are incorporated by reference in their entirety for all purposes to the same extent as if each individual publication, patent, patent application, and/or other document were individually indicated to be incorporated by reference for all purposes.
For reasons of completeness, various aspects of the invention are set out in the following numbered clauses:
Clause 1. A CRISPR/Cas-based genome editing system comprising: (a) a polynucleotide sequence encoding a guide RNA (gRNA) targeting a fragment of a mutant NF1 gene; (b) a polynucleotide sequence encoding a Cas protein or a fusion protein comprising the Cas protein; and (c) a polynucleotide sequence encoding a donor sequence comprising a fragment of a wild-type NF1 gene.
Clause 2. The system of clause 1, wherein the system comprises one or more vectors.
Clause 3. The system of clause 2, wherein the system comprises a first vector and a second vector, wherein the first vector comprises the polynucleotide sequence encoding the gRNA, and the polynucleotide sequence encoding the Cas protein or the fusion protein, and wherein the second vector comprises the polynucleotide sequence encoding the donor sequence.
Clause 4. The system of clause 3, wherein the polynucleotide sequence encoding the gRNA and the polynucleotide sequence encoding the Cas protein or the fusion protein are operably linked.
Clause 5. The system of any one of clauses 1-4, wherein the mutant NF1 gene comprises a mutation in the 5′ portion of the mutant NF1 gene, and wherein the polynucleotide sequence encoding the donor sequence further comprises a stop codon that is 5′ to the donor sequence.
Clause 6. The system of clause 5, wherein the gRNA targets a sequence upstream of the stop codon that is 5′ to the donor sequence and targets a sequence downstream of the donor sequence.
Clause 7. The system of clause 5 or 6, wherein the polynucleotide sequence encoding the donor sequence further comprises a promoter in between the stop codon and the donor sequence.
Clause 8. The system of clause 7, wherein the stop codon, the promoter, and the donor sequence are flanked on both ends (the 5′ and 3′ ends) with a sequence the gRNA targets.
Clause 9. The system of any one of clauses 5-8, wherein the stop codon, the donor sequence, and the 3′ portion of the mutant NF1 gene are in the same reading frame.
Clause 10. The system of any one of clauses 1-4, wherein the mutant NF1 gene comprises a mutation in the 3′ portion of the mutant NF1 gene, and wherein the polynucleotide sequence encoding the donor sequence further comprises a stop codon that is 3′ to the donor sequence.
Clause 11. The system of clause 10, wherein the gRNA targets a sequence upstream of the donor sequence and targets a sequence downstream of the stop codon that is 3′ to the donor sequence.
Clause 12. The system of clause 10 or 11, wherein the 5′ portion of the mutant NF1 gene, the donor sequence, and the stop codon are in the same reading frame.
Clause 13. The system of any one of clauses 5-12, wherein the gRNA targets a sequence flanking both sides of the polynucleotide sequence encoding the donor sequence and the stop codon.
Clause 14. The system of any one of clauses 1-13, wherein the donor sequence comprises multiple exons of the wild-type NF1 gene or a functional equivalent thereof.
Clause 15. The system of any one of clauses 1-14, wherein the donor sequence comprises one or more exons selected from exon 1, exon 2, exon 3, exon 4, exon 5, exon 6, exon 7, exon 8, exon 9, exon 10, exon 11, exon 12, exon 13, exon 14, exon 15, exon 16, exon 17, exon 18, exon 19, exon 20, exon 21, exon 22, exon 23, exon 24, exon 25, exon 26, exon 27, exon 28, exon 29, exon 30, exon 31, exon 32, exon 33, exon 34, exon 35, exon 36, exon 37, exon 38, exon 39, exon 40, exon 41, exon 42, exon 43, exon 44, exon 45, exon 46, exon 47, exon 48, exon 49, exon 50, exon 51, exon 52, exon 53, exon 54, exon 55, exon 56, and exon 57 of the wild-type NF1 gene or a functional equivalent thereof.
Clause 16. The system of clause 15, wherein the donor sequence comprises one or more contiguous exons of the wild-type NF1 gene or a functional equivalent thereof.
Clause 17. The system of any one of clauses 1-16, wherein the donor sequence comprises exons 1-30 of the wild-type NF1 gene, and wherein the gRNA targets a fragment of a mutant NF1 gene between exon 30 and exon 31.
Clause 18. The system of any one of clauses 1-17, wherein the gRNA comprises a polynucleotide sequence selected from SEQ ID NOs: 71-81 or a complement thereof or a truncation thereof.
Clause 19. The system of any one of clauses 1-17, wherein the gRNA is encoded by a polynucleotide sequence selected from SEQ ID NOs: 60-70 or a complement thereof or a truncation thereof, and/or hybridizes to a polynucleotide sequence selected from SEQ ID NOs: 49-59 or a complement thereof or a truncation thereof.
Clause 20. The system of any one of clauses 1-19, wherein the donor sequence comprises a polynucleotide sequence of SEQ ID NO: 82.
Clause 21. The system of any one of clauses 1-20, wherein the Cas protein is a Streptococcus pyogenes Cas9 protein or a Staphylococcus aureus Cas9 protein.
Clause 22. The system of clause 21, wherein the Cas protein comprises an amino acid sequence of SEQ ID NO: 20 or SEQ ID NO: 21.
Clause 23. The system of any one of clauses 2-22, wherein the vector is a viral vector.
Clause 24. The system of clause 23, wherein the vector is an Adeno-associated virus (AAV) vector.
Clause 25. The system of clause 24, wherein the AAV vector is AAV1, AAV2, AAV3, AAV4, AAV5, AAV6, AAV7, AAV8, AAV9, AAV-10, AAV-11, AAV-12, AAV-13, or AAVrh.74 vector.
Clause 26. The system of clause 24, wherein one of the one or more vectors comprises a polynucleotide sequence selected from SEQ ID NOs: 83-102.
Clause 27. The system of any one of clauses 1-26, wherein the molar ratio between the gRNA and the donor sequence is 1:1, or 1:5, or from 5:1 to 1:10, or from 1:1 to 1:5.
Clause 28. A cell comprising the system of any one of clauses 1-27.
Clause 29. A composition for restoring NF1 function in a cell having a mutant NF1 gene, the composition comprising the system of any one of clauses 1-27 or the cell of clause 28.
Clause 30. A kit comprising the system of any one of clauses 1-27, the cell of clause 28, or the composition of clause 29.
Clause 31. A method for restoring NF1 function in a cell or a subject having a mutant NF1 gene, the method comprising contacting the cell or the subject with the system of any one of clauses 1-27, the cell of clause 28, or the composition of clause 29.
Clause 32. The method of clause 31, wherein NF1 function is restored by inserting one or more wild-type exons of NF1 gene corresponding to the mutant NF1 gene.
SEQ ID NO: 1
(R = A or G; N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 2
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 3
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 4
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 5
(W = A or T; N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 6
(R = A or G; N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 7
(R = A or G; N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 8
(R = A or G; N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 9
(R = A or G; N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 10
(R = A or G; N can be any nucleotide residue, e.g., any of A, G, C, or T; V = A or C or G)
SEQ ID NO: 11
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 12
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 13
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 14
(R = A or G; N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 15
SEQ ID NO: 16
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 17
(N can be any nucleotide residue, e.g., any of A, G, C, or T)
SEQ ID NO: 18 DNA sequence of the gRNA constant region
SEQ ID NO: 19 RNA sequence of the gRNA constant region
SEQ ID NO: 20 Streptococcus pyogenes Cas9
SEQ ID NO: 21 Staphylococcus aureus Cas9
SEQ ID NO: 22 Streptococcus pyogenes Cas9 (with D10A)
SEQ ID NO: 23 Streptococcus pyogenes Cas9 (with D10A, H849A)
SEQ ID NO: 24 Polynucleotide sequence of D10A mutant of S. aureus Cas9
SEQ ID NO: 25 Polynucleotide sequence of N580A mutant of S. aureus Cas9
SEQ ID NO: 26 codon optimized polynucleotide encoding S. pyogenes Cas9
SEQ ID NO: 27 codon optimized nucleic acid sequences encoding S. aureus Cas9
SEQ ID NO: 28 codon optimized nucleic acid sequences encoding S. aureus Cas9
SEQ ID NO: 29 codon optimized nucleic acid sequence encoding S. aureus Cas9
SEQ ID NO: 30 codon optimized nucleic acid sequence encoding S. aureus Cas9
SEQ ID NO: 31 codon optimized nucleic acid sequence encoding S. aureus Cas9
SEQ ID NO: 32 codon optimized nucleic acid sequences encoding S. aureus Cas9
SEQ ID NO: 33 codon optimized nucleic acid sequences encoding S. aureus Cas9
SEQ ID NO: 34 Vector (pDO242) encoding codon optimized nucleic acid sequence encoding S. aureus Cas9
SEQ ID NO: 35 SV40 NLS (Pro-Lys-Lys-Lys-Arg-Lys-Val)
SEQ ID NO: 82 Polynucleotide donor sequence
SEQ ID NO: 83 (Plasmid 16) Polynucleotide sequence of the donor sequence flanked by gRNA 1 target sites (7472 bp)
SEQ ID NO: 84 (Plasmid 47) Polynucleotide sequence of the donor sequence flanked by gRNA 3 target sites (7465 bp)
SEQ ID NO: 85 (Plasmid 48) Polynucleotide sequence of the donor sequence flanked by gRNA 4 target sites (7472 bp)
SEQ ID NO: 86 (Plasmid 49) Polynucleotide sequence of the donor sequence flanked by gRNA 6 target sites (7474 bp)
SEQ ID NO: 87 Polynucleotide sequence of gRNA 1 in AAV vector (7450 bp)
SEQ ID NO: 88 Polynucleotide sequence of gRNA 3 in AAV vector (7450 bp)
SEQ ID NO: 89 Polynucleotide sequence of gRNA 4 in AAV vector (7451 bp)
SEQ ID NO: 90 Polynucleotide sequence of gRNA 6 in AAV vector (7451 bp)
SEQ ID NO: 91 Polynucleotide sequence of gRNA 1 in a plasmid cloning vector pDO240, used for evaluating editing efficiency with Surveyor Assay, TIDE, and next-generation sequencing assays (3235 bp)
SEQ ID NO: 92 Polynucleotide sequence of gRNA 2 in a plasmid cloning vector (3236 bp)
SEQ ID NO: 93 Polynucleotide sequence of gRNA 3 in a plasmid cloning vector (3235 bp)
SEQ ID NO: 94 Polynucleotide sequence of gRNA 4 in a plasmid cloning vector (3236 bp)
SEQ ID NO: 95 Polynucleotide sequence of gRNA 5 in a plasmid cloning vector (3237 bp)
SEQ ID NO: 96 Polynucleotide sequence of gRNA 6 in a plasmid cloning vector (3236 bp)
SEQ ID NO: 97 Polynucleotide sequence of gRNA 7 in a plasmid cloning vector (3237 bp)
SEQ ID NO: 98 Polynucleotide sequence of gRNA 8 in a plasmid cloning vector (3237 bp)
SEQ ID NO: 99 Polynucleotide sequence of gRNA 9 in a plasmid cloning vector (3236 bp)
SEQ ID NO: 100 Polynucleotide sequence of gRNA 10 in a plasmid cloning vector (3237 bp)
SEQ lD NO: 101 Polynucleotide sequence of gRNA 11 in a plasmid cloning vector (3237 bp)
SEQ lD NO: 102 (Plasmid 39) Polynucleotide sequence of the donor sequence flanked by scrambled gRNA target sites (7472 bp)
This application claims priority to U.S. Provisional Pat. Application No. 63/015,740, filed Apr. 27, 2020, and U.S. Provisional Pat. Application No. 63/015,866, filed Apr. 27, 2020, each of which is incorporated herein by reference in its entirety.
| Filing Document | Filing Date | Country | Kind |
|---|---|---|---|
| PCT/US2021/029500 | 4/27/2021 | WO |
| Number | Date | Country | |
|---|---|---|---|
| 63015866 | Apr 2020 | US | |
| 63015740 | Apr 2020 | US |
