CA2291512A1 - Methods of making an rnp particle having nucleotide integrase activity - Google Patents

Methods of making an rnp particle having nucleotide integrase activity Download PDF

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CA2291512A1
CA2291512A1 CA002291512A CA2291512A CA2291512A1 CA 2291512 A1 CA2291512 A1 CA 2291512A1 CA 002291512 A CA002291512 A CA 002291512A CA 2291512 A CA2291512 A CA 2291512A CA 2291512 A1 CA2291512 A1 CA 2291512A1
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intron
group
rna
sequence
nucleotide
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Alan M. Lambowitz
Georg Mohr
Roland Saldanha
Manabu Matsuura
Clifford James Beall
Jian Yang
Huatao Guo
Steven Zimmerly
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Ohio State University Research Foundation
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Abstract

Methods for preparing nucleotide integrases are provided. The nucleotide integrases are prepared by combining in vitro an excised, group II intron RNA, referred to hereinafter as "exogenous RNA", with a group II intron-encoded protein. The exogenous RNA is prepared by in vitro transcription of a DNA molecule which comprises a group II intron sequence.

Description

METHODS OF MAKING AN RNP PARTICLE
HAVING NUCLEOTIDE INTEGRASE ACTIVITY
BACKGROUND
Nucleotide integrases are molecular complexes that are capable of cleaving nucleic acid substrates at specific recognition sites and of concomitantly inserting nucleic acid molecules into the nucleic acid substrate at the cleavage site. Thus, nucleotide integrases are useful tools, particularly for genome mapping, genetic engineering and disrupting the synthesis of gene products. Structurally, nucleotide integrases are ribonucleoprotein (RNP) particles that comprise an excised, group II intron RNA and a group II intron-encoded protein, which is bound to the group II intron RNA.
Conventionally, nucleotide integrases are made by isolating RNP particles that have nucleotide integrase activity from source organisms which comprise a DNA
molecule that encodes both the RNA and protein subunits of the nucleotide integrase. In order to obtain nucleotide integrases other than wild type, the source organisms are mutagenized. The mutagenesis is a laborious, multistep process. Moreover, this process yields limited quantities of the nucleotide integrase.
Accordingly, it is desirable to have methods for making nucleotide integrases which are not laborious and which permit the nucleotide integrase to be readily modified from the wild type. Methods which yield at least microgram quantities of substantially pure nucleotide integrases are especially desirable.
SUMMARY OF THE INVENTION
The present invention provides new, improved, and easily manipulable methods for making nucleotide integrases.
In one embodiment, the nucleotide integrase is prepared by introducing a DNA
molecule which comprises a group II intron DNA sequence into a host cell.
Preferably the DNA molecule further comprises a sequence which encodes a tag that facilitates isolation of RNP particles having nucleotide integrase activity from the host cell.
Preferably, the tag sequence is linked to the open reading frame (ORF) sequence of the group II
intron DNA.
The group II intron DNA sequence is then expressed in the host cell such that RNP particles having nucleotide integrase activity are formed in the cell. Such RNP
particles comprise an excised group II intron RNA molecule and a group II intron-encoded protein, both of which SUBSTITUTE SHEET (RULE 26) are encoded by the introduced DNA molecule. Thereafter, the RNP particles having nucleotide integrase activity are isolated from the cell.
In another embodiment, the nucleotide integrase is prepared by combining in vitro an excised, group II intron RNA, referred to hereinafter as "exogenous RNA", with a group II
intron-encoded protein. The exogenous RNA is prepared by in vitro transcription of a DNA
molecule which comprises a group II intron sequence. The group II intron-encoded protein is made by introducing into a host cell a DNA molecule that comprises at least the open reading frame sequence of a group II intron and then expressing the open reading frame sequence in the host cell. The DNA molecule may comprise the open reading frame sequence operably linked to a promoter, preferably an inducible promoter. Thereafter, the cell is fractionated and the protein is recovered and combined in vitro with the exogenous RNA to provide RNP
particles having nucleotide integrase activity. Alternatively, the DNA
molecule may comprise a group II intron sequence that encodes both a group II intron RNA as well as a group II intron encoded protein. The DNA molecule is then expressed in the host cell to 1 S provide RNP particles that comprise the group II intron-encoded protein bound to the group II
intron RNA. Thereafter, the RNP particles comprising the group II intron-encoded protein and the group II intron RNA are isolated from the cell and treated with a nuclease to remove the RNA and to provide the group II-intron encoded protein. The group II
intron-encoded protein is then combined in vitro with the exogenous RNA to provide RNP
particles having nucleotide integrase activity.
The present invention also relates to isolated RNP particles having nucleotide integrase activity.
BRIEF DESCRIPTION OF THE DRAWINGS
Figure 1 depicts the interaction at the target site between the EBS 1 and EBS2 sequences of the group II intron RNA 2 of the S. cerevisiae mitochondrial COXI gene, hereinafter referred to as the "aI2" RNA, with the IBS1 and IBS2 sequences of a nucleic acid substrate. The cleavage site is represented by an arrow.
Figure 2 is a schematic representation of the domains in three representative group II
intron encoded proteins, namely the protein which is encoded by the ORF
sequence of the group II intron 2 of the S. cerevisiae mitochondria) COXI gene, the group II
intron 2 of the SUBSTITUTE SHEET (RULE 26) M. polymorpha mitochondria) COXl gene, and the group II intron 1 of the N.
tabacum chloroplast trnK gene.
Figure 3 is the plasmid map of pETLtrAl9.
Figure 4 shows the nucleotide sequence of the 2.8 kb HindIII fragment that is present in pETLtrAl9 and that includes the Ll.ItrB intron DNA sequence and portions of the nucleotide sequence of the flanking exons ltrBEl and ltrBE2, SEQ. ID. NO. 1., the nucleotide sequence of the LtrA open reading frame, SEQ. ID. ND. 2, and the amino acid sequence of the LtrA protein, SEQ. ID. NO. 3.
Figure 5 is the plasmid map of plasmid pETLtrAI-1.
Figure 6 is a schematic representation of the inserts in pLEl2, pETLtrAl9 and pETLtrAI-1.
Figure 7A is the sequence of the sense strand of a double-stranded DNA
substrate, SEQ. ID. NO. 4, which is cleaved by RNP particles that comprise a wild-type excised, LLItrB intron RNA and an LtrA protein. Figure 7B is the sequence of the sense strand of a 1 S double stranded DNA substrate which is cleaved by RNP particles that comprise an excised Ll.ItrB intron RNA having a modified EBS I sequence and an LtrA protein.
Figure 8a is a schematic depiction of the substrate which is cleaved by RNP
particles comprising the wild-type Ll.ltrB intron RNA and the LtrA protein, and Figure 8b shows the IBS 1 and IBS2 sequences of the substrate and the cleavage sites of the double-stranded DNA
substrate which is cleaved by these RNP particles.
DETAILED DESCRIPTION OF THE INVENTION
Nucleotide InteQrases Functionally, nucleotide integrases are endonucleases that are capable of cleaving nucleic acid substrates at specific recognition sites and of concomitantly inserting nucleic acid molecules into the substrate at the cleavage site. Structurally, nucleotide integrases are ribonucleoprotein (RNP) particles that comprise an excised, group II intron RNA and a group II intron-encoded protein, which is bound to the excised group II intron RNA.
"Excised group II intron RNA," as used herein, refers to the RNA that is, or that is derived from, an in vitro or in vivo transcript of the group II intron DNA and that lacks flanking exon sequences at the 5' end and the 3' end of the intron sequence. The excised, group II
intron RNA
typically has six domains and a characteristic secondary and tertiary structure, which is SUBSTITUTE SHEET (RULE 26) shown in Saldahana et al., 1993, Federation of the American Society of Experimental Biology Journal, Vol 7 p15-24, which is specifically incorporated herein by reference.
Domain IV of the group II intron RNA contains the open reading frame ("ORF") nucleotide sequence which encodes the group II intron encoded protein. The excised group II intron RNA
also has two sequences in domain I which are capable of hybridizing with two sequences in the target site of the intended nucleic acid substrate. The first sequence, referred to hereinafter as the "EBS 1" sequence, is capable of hybridizing with a sequence, referred to hereinafter as the "IBS1" sequence, which is immediately upstream of the cleavage site in the substrate. The second sequence, referred to hereinafter as the "EBS2" sequence, is capable of hybridizing with a sequence, hereinafter referred to as the "IB S2" sequence, which is upstream of the IBS 1 sequence.
The excised group II intron RNA has a wild-type sequence, i.e. a sequence which is identical to the sequence of a group II intron RNA that is found in nature, or the excised group II intron RNA has a modified sequence, i.e. a sequence which is different from the sequence of group II intron RNA molecules that are found in nature. For nucleotide integrases in which the group II intron RNA has a wild-type sequence, the EBSI sequence typically is complementary to a sequence of about 5-7 nucleotides, hereinafter referred to as the "first set" , which is located at the 3' end of the exon that is joined to the 5' end of the intron in the gene.
Similarly, the EBS2 sequence of the wild-type group II intron RNA typically is complementary to a sequence of about 5-7 nucleotides in the 5' exon, hereinafter referred to as the "second set" , which is upstream, typically immediately upstream, of the first set. Thus, the EBS1 and EBS2 sequences of a wild-type group II intron RNA can usually be predicted by finding sequences in domain I of the intron that are complementary to the first set and second set of nucleotides in the 5' exon.
In the wild-type group II intron RNA of the Lactococcus lactis ItrB gene, hereinafter referred to as the wild-type Ll.ItrB intron RNA, EBS1 comprises 7 nucleotides, is located at position 3132-3138 (numbered according to Mills et al., 1996, J. Bact., 178, 3531-3538), and has the sequence GUUGUGG. EBS2 of the wild-type Ll.ltrB intron RNA comprises 6 nucleotides, is located at positions 3076-3081 and has the sequence AUGUGU. In the wild-type group II intron RNA 1 of the S. cerevisiae mitochondrial COXl gene, hereinafter referred to as the "wild-type all RNA", EBS1 comprises 6 nucleotides, is located at position (numbered according to Bonitz et aL, 1980, J. Biol. Chem.: 255, 11927-11941), and has the SUBSTITUTE SHEET (RULE 26) sequence CGUUGA. EBS2 of the wild-type aI l RNA comprises 6 nucleotides, is located at positions 376-381 and has the sequence ACAAUU. In the wild-type group II
intron RNA 2 of the S. cerevisiae mitochondrial C'OXI gene, hereinafter referred to as the "wild-type aI2" RNA, EBS 1 comprises 6 nucleotides, is located at position 2985-2990 (numbered according to Bonitz S et al., 1980, J. Biol. Chem.: 2SS, 11927-11941) and has the sequence AGAAGA.
EBS2 of the wild-type aI2 RNA comprises 7 nucleotides, is located at positions 2935-29410, and has the sequence UCAUUAA. The interaction between EBS1 and EBS2 of the wild-type aI2 RNA
with its intended substrate is depicted in Figure 1.
The excised group II intron RNA may also have a sequence different from a group II
intron RNA that is found in nature, and thus be a modified, excised group II
intron RNA.
Modified excised group II intron RNA molecules, include, for example, group II
intron RNA
molecules that have nucleotide base changes or additional nucleotides in the internal loop regions of the group II intron RNA, preferably the internal loop region of domain IV and group II intron RNA molecules that have nucleotide base changes in the sequences of EBS 1 and/or 1 S EBS2. Nucleotide integrases in which the group II intron RNA has nucleotide base changes in the sequences of EBS1 or EBS2, as compared to the wild type, typically have altered specificity for the intended nucleic acid substrate.
The group II intron-encoded protein has an X domain, a reverse transcriptase domain, and, preferably, a Zn domain. The X domain of the protein has a maturase activity. The Zn domain of the protein has Zn'' finger-like motifs. As used herein, a group II
intron-encoded protein includes modified group II intron-encoded proteins that have additional amino acids at the N terminus, or C terminus, or alterations in the internal regions of the protein as well as wild-type group II intron-encoded proteins. The domains 'of three representative group I1 intron-encoded proteins are depicted in Figure 2.
2S The RNP particles having nucleotide integrase activity cleave single-stranded RNA
molecules, single-stranded DNA molecules, and double-stranded DNA molecules.
The RNP
particles having nucleotide integrase activity also insert the group II intron RNA subunit of the RNP particle into the cleavage site. Thus, RNP particles having nucleotide integrase activity both cleave nucleic acid substrates and insert nucleic acid molecules into the cleavage site. With double-stranded DNA substrates, the nucleotide integrase inserts the group II intron RNA into the first strand, i.e., the strand that contains the IBS1 and IBS2 sequences, of the cleaved DNA substrate and, preferably, a cDNA molecule into the second strand of the SUBSTITUTE SHEET (RULE 26) cleaved DNA substrate. The excised group II intron RICA subunit of the nucleotide integrase catalyzes cleavage of the single-stranded-substrates and the first strand of the double-stranded DNA substrate. The cleavage that is catalyzed by the excised group II
intron RNA also results in the insertion, either partially or completely, of the excised group II intron RNA into s the cleavage site, i.e. between nucleotide +1, which is immediately downstream of the cleavage site, and nucleotide -l, which is immediately upstream of the cleavage site.
The group II intron-encoded protein subunit catalyzes cleavage of the second strand of the double-stranded DNA
substrate. The second strand of the double stranded DNA substrate is cut at a position from about 9 to about 11 base pairs downstream of the cleavage site in the first strand, i.e. at a site between nucleotide positions +9, +10, and +11. It is believed that the group II intron-encoded protein also assists cleavage of the first strand of the double stranded DNA
substrate by stabilizing the group II intron RNA. Thus, the RNP particle having nucleotide integrase activity is active under conditions that are similar to physiological conditions.
To cleave the substrates, it is preferred that the EBSI and EBS2 sequences of the group II intron RNA of the nucleotide integrase have at least 90% complementarity, preferably full complementarity, with the IBSI and IBS2 sequences, respectively, of the intended substrate.
Thus, if there is not at least 90% complementarity between the EBS sequences of the excised group II intron RNA and IBS sequences of the intended substrate, it is preferred that nucleotide base changes be made in the non-complementary EBS sequences. To cleave single-stranded and double-stranded nucleic acid substrates efficiently, it is preferred that the nucleotide delta, which immediately precedes the first nucleotide of EBS1 be complementary to the nucleotide at +1 in the target site. Thus, if the delta nucleotide is not complementary to the nucleotide at +1 in the target site, the group II intron RNA is modified to contain a delta nucleotide which is complementary to the nucleotide at +I on the sense strand of the substrate. To cleave double stranded DNA substrates efficiently, it is preferred that the target site has a sequence that is recognized by the group II intron-encoded protein of the nucleotide integrase.
For example, cleavage of a double-stranded DNA substrate is achieved with a nucleotide integrase comprising a wild-type Ll.ltrB RNA and LtrA protein if the first strand of the substrate contains the sequence, 5'-TCGATCGTGAACACATCCATAACC'3', SEQ.ID.NO.- which represents the sequence from -23 to +1 in the target site of the first strand.
SUBSTITUTE SHEET (RULE 26) A. Preparation of the Nucleotide Integrase b~~solation from a Genetically Engineered Cell.
In one embodiment, RNP particles having nucleotide integrase activity are made by introducing an isolated DNA molecule which comprises a group II intron DNA
sequence into a host cell. Preferably, the DNA molecule further comprises an IBS 1 sequence and an IBS2 sequence just upstream of the 5' end of the group II intron DNA sequence to allow splicing of the group II intron RNA from a transcript of the group II intron DNA
sequence. Suitable DNA molecules include, for example, viral vectors, plasmids, and linear DNA
molecules.
Following introduction of the DNA molecule into the host cell, the group II
intron DNA
sequence is expressed in the host cell such that excised RNA molecules encoded by the introduced group II intron DNA sequence and protein molecules encoded by introduced group II intron DNA sequence are formed in the cell. The excised group II
intron RNA and group II intron-encoded protein are combined within the host cell to produce an RNP particle having nucleotide integrase activity.
Preferably, the introduced DNA molecule also comprises a promoter, more preferably an inducible promoter, operably linked to the group II intron DNA sequence.
Preferably, the DNA molecule further comprises a sequence which encodes a tag to facilitate isolation of the RNP particles having nucleotide integrase activity, such as, for example, an affinity tag and/or an epitope tag. Preferably, the tag sequences are at the 5' or 3' end of the open reading frame sequence. Suitable tag sequences include, for example, sequences which encode a series of histidine residues, the Herpes simplex glycoprotein D, i.e., the HSV
antigen, or glutathione S-transferase. An especially suitable tag is a sequence which encodes the intein from the S. cerevisiae VMA1 gene linked to the chitin binding domain from Bacillus circulars. Typically, the introduced DNA molecule also comprises nucleotide sequences that encode a replication origin and a selectable marker. Optionally, the introduced DNA
molecule comprises sequences that encode molecules that modulate expression, such as for example T7 lysozyme.
The DNA molecule comprising the group II intron sequence is introduced into the host cell by conventional methods, such as, by cloning the DNA molecule into a vector and by introducing the vector into the host cell by conventional methods, such as electroporation or by CaClz-mediated transformation procedures. The method used to introduce the DNA
molecule depends on the particular host cell used. Suitable host cells are those which are SUBSTITUTE SHEET (RULE 26) capable of expressing the group II intron DNA sequence. Suitable host cells include, for example, heterologous or homologous bacterial cells, yeast cells, mammalian cells, and plant cells. In those instances where the host cell genome and the group II intron DNA sequence use different genetic codes, it is preferred that the group II intron DNA
sequence be modified to comprise codons that correspond to the genetic code of the host cell. The group II intron DNA sequence, typically, is modified by using a DNA synthesizer or by in vitro site directed mutagenesis, such as by PCR mutagenesis, to prepare a group II intron DNA
sequence with different codons. Alternatively, to resolve the differences in the genetic code of the intron and the host cell, DNA sequences that encode the tRNA molecules which correspond to the genetic code of the group II intron are introduced into the host cell.
Optionally, DNA
molecules which comprise sequences that encode factors that assist in RNA or protein folding, or that inhibit RNA or protein degradation are also introduced into the cell.
The DNA sequences of the introduced DNA molecules are then expressed in the host cell to provide a transformed host cell. As used herein the term "transformed cell" means a host cell that has been genetically engineered to contain and express additional DNA, primarily heterologous DNA, and is not limited to cells which are cancerous.
Then the RNP
particles having nucleotide integrase activity are isolated from the transformed host cells.
The RNP particles having nucleotide integrase activity are isolated, preferably by lysing the transformed cells, such as by mechanically and/or enzymatically disrupting the cell membranes of the transformed cell. Then the cell lysate is fractionated into an insoluble fraction and soluble fraction. Preferably, an RNP particle preparation is isolated from the soluble fraction. The RNP particle preparations include the RNP particles having nucleotide integrase activity as well as ribosomes, mRNA and tRNA molecules. Suitable methods for isolating RNP particle preparations include, for example, centrifugation of the soluble fraction through a sucrose cushion. The RNP particles, preferably, are further purified from the RNP particle preparation or from the soluble fraction by, for example, separation on a sucrose gradient, or a gel filtration column, or by other types of chromatography. For example, in those instances where the group II-intron encoded protein subunit of the desired RNP particle has been engineered to include a tag, the RNP particles having nucleotide integrase activity are purified from the particle preparation by affinity chromatography on a matrix which recognizes and binds to the tag. For example, NiNTA SuperflowTH
from Qiagen, Chatsworth CA, is suitable for isolating RNP particles having nucleotide integrase SUBSTITUTE SHEET (RULE 26) activity when the group II intron-encoded protein has a histidine tag. It has been found that the a system which employs a chitin column and an intein and chitin binding domain tag on the group II intron-encoded protein results in the production of RNP particles that are substantially pure, i.e., the intron encoded protein represents at least 95%
of the protein in the RNP particles eluted from the column. Thus, the latter system is particularly suitable for isolating RNP particles having nucleotide integrase activity.
B. Prenaration of the Nucleotide lntegrase by Combining- Exogenous RNA with a Group II Intron-Encoded Protein to Form a Reconstituted RNP Particle In another embodiment, the nucleotide integrase is formed by combining an isolated exogenous RNA with an isolated group II intron-encoded protein in vitro to provide a reconstituted RNP particle having nucleotide integrase activity. The exogenous RNA is made by in vitro transcription of the group II intron DNA. The exogenous RNA may be made by in vitro transcription of the group II intron DNA only, i.e. the transcript lacks flanking exon sequences. Alternatively, the exogenous RNA is made by in vitro transcription of the group II intron DNA and the DNA of all, or portions, of the flanking exons to produce an unprocessed transcript which contains the group II intron RNA and the RNA
encoded by the flanking exons or portions thereof. Then the exogenous RNA is spliced from the unprocessed transcript.
The purified group II intron-encoded protein is prepared by introducing into a host cell an isolated DNA molecule that comprises at least the open reading frame sequence of a group II intron. The DNA molecule may comprise a group II intron ORF sequence operably linked to an inducible promoter. Alternatively, the DNA molecule may comprise a group II
intron DNA sequence. Preferably, the introduced DNA molecule also comprises a sequence at the 5' or 3' end of the group II intron ORF sequence which, when expressed in the host cell, provides an affinity tag or epitope on the N-terminus or C-terminus of the group II
intron-encoded protein. Thus, the DNA molecule may comprise at the 5' or 3' end of the ORF, for example, a sequence which encodes a series of histidine residues, or the HSV
antigen, glutathione-S-transferase, or an intein linked to a chitin binding domain. Typically, the DNA molecule also comprises nucleotide sequences that encode a replication origin and a selectable marker.
SUBSTITUTE SHEET (RULE 26) When the introduced DNA molecules comprise a group II intron ORF sequence operably linked to an inducible promoter, the ORF sequence is then expressed in the host cell preferably by adding a molecule which induces expression, to provide a host cell that contains RNP particles comprising the group II intron-encoded protein associated with endogenous nucleic acids, particularly endogenous RNA molecules. Then the transformed cell is lysed, and preferably fractionated into a soluble fraction and an insoluble fraction. The RNP particles comprising the protein and the endogenous RNA are then isolated, preferably from the soluble fraction, preferably by using methods such as affinity chromatography. The RNP particles are then incubated with the exogenous RNA, preferably in a buffer, to allow the exogenous RNA to displace the associated RNA molecules and to form RNP
particles having nucleotide integrase activity. Optionally, the RNP particles, are treated with a nuclease to remove the RNA that is associated with the group II intron encoded protein prior to incubation of the protein preparation with the exogenous RNA. The RNP
particles may be treated with the nuclease by adding the nuclease to the soluble fraction.
Alternatively, the RNP particles may be treated with the nuclease after isolation of the RNP
particles from the soluble fraction.
When DNA molecules comprise a splicing-competent group II intron sequence, are introduced and expressed in the host cells, RNP particles comprising a group II intron-encoded protein associated with an excised group II intron RNA that encodes the protein are produced. When DNA molecules comprise a splicing-defective group II intron sequence, are introduced and expressed in the host cells, the group II intron-encoded protein is not associated with an excised, group II intron RNA that encodes the protein The RNP particles that are produced when a splicing-defective group II intron DNA sequence is introduced and expressed in a host cell comprise other types of RNA molecules, such as for example, unspliced group II intron RNA molecules that encode the protein, ribosomal RNA
molecules, mRNA molecules, tRNA molecules or other nucleic acids. Following formation of the RNP
particles in the host cell, the transformed cell is lysed, and preferably fractionated into a soluble fraction and an insoluble fraction. The RNP particles comprising the protein are then isolated, preferably from the soluble fraction, preferably by using methods such as affinity chromatography. The isolated RNP particles are then treated with a nuclease that degrades all of the endogenous RNA molecules. Preferably the RNP particles are treated with a nuclease which can be chemically inactivated, such as for example, micrococcal nuclease. The group SUBSTITUTE SHEET (RULE 26) _ .

II intron-encoded protein preparation is then combined with the exogenous RNA, preferably in a buffer, to allow formation of RNP particles having nucleotide integrase activity These methods enable production of increased quantities of nucleotide integrases.
Conventional methods produce approximately 0.1 to 1 ~g of an RNP particles having nucleotide integrase per liter of cultured cells. However, these RNP particles are highly contaminated with other proteins. The methods of the present invention enable the production of at least 0.5 mg of RNP particles having nucleotide integrase activity per liter of cultured cells. Moreover, the RNP particles having nucleotide integrase activity produced in accordance with the present methods are substantially pure, i.e., at least 95%
of the protein in the final RNP particle preparation is the group II intron-encoded protein. The present methods also offer the further advantage of permitting the sequences of the RNA
component and the protein component of the nucleotide integrase to be readily modified.
Typically, the nucleotide integrases are modified by introducing nucleotide base changes, deletions, or additions into the group II intron RNA by PCR mutagenesis of the group II
intron.
The following examples of methods for preparing a group II intron-encoded protein and for preparing nucleotide integrases are included for purposes of illustration and are not intended to limit the scope of the invention.
Preparing Nucleotide Inte~rases By Coexpression of a Group II Intron RNA and a Group II
Intron Encoded Protein Example 1 RNP particles having nucleotide integrase activity and comprising an excised RNA
that is encoded by the Ll.ltrB intron of a lactococcal cojugative element pRS01 of Lactococcus lactic and the protein encoded by the ORF of the~Ll.ltrB intron were prepared by transforming cells of the BLR(DE3) strain of the bacterium Escherichia coli, which has the recA genotype, with the plasmid pETLtrAl9. Plasmid pETLtrAl9, which is schematically depicted in Figure 3, comprises the DNA sequence for the group II intron Ll.ltrB from Lactococcus lactic, shown as a thick line, positioned between portions of the flanking exons ltrBEl and ItrBE2, shown as open boxes. pETLtrAl9 also comprises the DNA
sequence for the T7 RNA polymerase promoter and the T7 transcription terminator. The sequences are oriented in the plasmid in such a manner that the ORF sequence, SEQ. ID. NO.
2, within the Ll.ltrB intron is under the control of the T7 RNA polymerase promoter. The ORF
of the LLItrB intron, shown as an arrow box, encodes the protein LtrA. The sequence of the Ll.ltrB

SUBSTITUTE SHEET (RULE 26) intron and the flanking exon sequences present in pETLtrAl9 are shown in Figure 4 and SEQ.
ID. NO. I . Vertical lines in Figure 4 denote the junctions between the intron and the flanking sequences. The amino acid sequence of the LtrA protein, SEQ. ID. NO. 3 is shown under the ORF sequence, SEQ. ID. NO. 2, in Figure 4. The sequences of EBSI and EBS2 include nucleotides 457 through 463 (EBS1), nucleotides 401 through 406 (EBS2a) , and nucleotides 367 through 372 (EBS2b). Domain IV is encoded by nucleotide 705 to 2572.
pETLtrAl9 was prepared first by digesting pLE 12, which was obtained from Dr.
Gary Dunny from the University of Minnesota, with HindIII and isolating the restriction fragments on a 1 % agarose gel. A 2.8 kb HindIII fragment which contains the LLItrB
intron together with portions of the flanking exons ItrBEI and ItrBE2 was recovered from the agarose gel and the single-stranded overhangs were filled in with the Klenow fragment of DNA
polymerase I
obtained from Gibco BRL, Gaithersburg, MD. The resulting fragment was ligated into plasmid pET-l la that had been digested with XbaI and treated with Klenow fragment. pET-11 a was obtained from Novagen, Madison, WI.
pETLtrAl9 was introduced into the E. coli cells using the conventional CaCI,-mediated transformation procedure of Sambrook et al. as described in "Molecular Coning A
Laboratory Manual", pages 1-82, 1989 . Single transformed colonies were selected on plates containing Luria-Bertani (LB) medium supplemented with ampicillin to select the plasmid and with tetracycline to select the BLR strain. One colony was inoculated into 2 ml of LB
medium supplemented with ampicillin and grown overnight at 37°C with shaking. 1 ml of this culture was inoculated into 100 ml LB medium supplemented with ampicillin and grown at 37°C with shaking at 200 rpm until OD5~5 of the culture reached 0.4.
Then isopropyl-beta-D-thiogalactoside was added to the culture to a final concentration of 1 mM
and incubation was continued for 3 hours. Then the entire culture was harvested by centrifugation at 2,200 x g, 4°C, for 5 minutes. The bacterial pellet was washed with 150 mM NaCI
and finally resuspended in 1/20 volume of the original culture in 50 mM Tris, pH 7.5, 1 mM
EDTA, 1 mM DTT, and 10% (v/v) glycerol (Buffer A)and 2 mg/ml lysozyme. Bacteria were frozen at -70°C.
To produce a lysate the bacteria were thawed and frozen at -70°C three times. Then 4 volumes of 500 mM KCI, 50 mM CaCI,, 25 mM Tris, pH 7. 5, and 5 mM DTT (HKCTD) were added to the lysate and the mixture was sonicated until no longer viscous, i.e. for about 5 seconds or longer. The lysate was fractionated into a soluble fraction and insoluble fraction SUBSTITUTE SHEET (RULE 26) by centrifugation at 14,000 x g, 4°C, for 1 S minutes. Then 5 ml of the resulting supernatant, i.e., the soluble fraction, were loaded onto a sucrose cushion of 1.85 M
sucrose in HKCTD
and centrifuged for 17 hours at 4°C, 50,0000 rpm in a Ti 50 rotor from Beckman. The pellet which contains the RNP particles was washed with 1 ml water and then dissolved in 25 ~1 10 mM Tris, pH 8. 0, 1 mM DTT on ice. Insoluble material was removed by centrifugation at 15, 000 x g, 4°C, for 5 minutes. The result is a preparation of partially-purified RNP particles that comprise the excised Ll.ltrB intron RNA and the LtrA protein The yield of RNP particles was 25 to 50 O.D.,bo units ( ~ 16 ~g protein) per 100 ml culture, with 1 O.D.ZGO units of RNPs containing 0.3 to 3 pg LtrA protein. To minimize nuclease activity, the partially-purified RNPs were further purified by an additional centrifugation through a 1.85 M sucrose cushion, as described above.
Example 2 RNP particles having nucleotide integrase activity and comprising the LtrA
protein and the excised Ll.ltrB intron RNA were prepared as described in example 1 except the plasmid pETLtrAl9 was used to transform cells of the BL21(DE3) strain of E.
coli. The transformed cells were fractionated into a soluble fraction and an insoluble fraction as described in Example 1 to provide a preparation of RNP particles having nucleotide integrase activity Example 3 RNP particles having nucleotide integrase activity and comprising the LtrA
protein and the excised Ll.ltrB intron RNA were prepared by transforming cells of the E. coli strains BLR(DE3) with gETLtrAl9 as described in Example I except that the transformed E. coli were grown in SOB medium and shaken at 300 rpm during the 3 hour incubation.
The transformed cells were fractionated into a soluble fraction and an insoluble fraction as described in Example 1 to provide a preparation of RNP particles having nucleotide integrase activity Example 4 RNP particles having nucleotide integrase and comprising the LtrA protein and the excised Ll.ltrB intron RNA were prepared as described _above in sample 1 except that the plasmid pETLtrAl9 was used to transform cells of the E. coli strain BL21(DE3).
The cells SUBSTITUTE SHEET (RULE 26) were also transformed with plasmid pOM62 which is based on the plasmid pACYC184 and has an approximately 150 by insert of the argU(dnaY) gene at the EcoRI site.
The argU gene encodes the tRNA for the rare arginine codons AGA and AGG. The LtrA gene contains 17 of the rare arginine codons. The transformed cells were grown in SOB medium and fractionated into a soluble fraction and an insoluble fraction as described in Example 1 to provide a preparation of RNP particles having nucleotide integrase activity.
Example 5 RNP particles having nucleotide integrase and comprising the excised LLItrB
intron RNA and the LtrA protein were prepared by transforming host cells as described above in Example 1 except that the LtrA ORF was tagged at the C-terminus with a Hisb affinity tag and an epitope derived from the Herpes simplex virus glycoprotein D. The tag is used to facilitate isolation of the RNP particles. The plasmid adding the tags was made in two steps by using PCR. In the first step, a fragment containing exon 1 and the LtrA ORF
was 1 ~ amplified using primers LtrAexl.Xba having the sequence 5' TCACCTCATCTAGACATTTTCTCC 3', SEQ. ID. NO. 5 which introduces an Xba I site in exon 1 of LtrB, and LtrAexpr3 5'CGTTCGTAAAGCTAGCCTTGTGTTTATG 3', SEQ. ID.
NO. 6, which substitutes a CGA (arginine) codon for the stop codon and introduces an Nhe I
site at the 3' end of the LtrA ORF. The PCR product was cut with XbaI and Nhe I, and the restriction fragments gel purified and cloned into pET-27b(+), cut with Xba I
and Nhe I
obtained from Novagen, Madison, WI. The resulting plasmid pIntermediate-C
fuses the 3' end of the LtrA ORF to an HSV tag and Hisb purification tag, both of which are present on the vector pET-27b(+). In a second step, intron sequences 3' to the ORF and exon 2 are amplified using pLEl2 as a template and the 5' primer LtrAConZnl, having the sequence 5'CACAAGTGATCATTTACGAACG 3', SEQ. ID. No. 7 and the 3' primer LtrAex2, which has the sequence 5'TTGGGATCCTCATAAGCTTT GCCGC 3', SEQ. ID. NO. 8. The PCR
product is cut with BcII and BamHI, the resulting fragment filled in, gel purified and cloned into pIntermediate-C, which has been cleaved with Bpu1102I and filled in. The resulting plasmid is designated pC-hisLtrAl9.
Cells of the BLR(DE3) strain of E. coli were transformed as described in example 1 with pIntermediate-C and cultured at 37°C for 3 hours in SOB medium as described in example 3. The cells were also fractionated into a soluble fraction, which contains RNP

SUBSTITUTE SHEET (RULE 26) particles having nucleotide integrase activity, and an insoluble fraction as described in example 1. The RNP particles were further purified as described in example 1.

RNP particles having nucleotide integrase activity and comprising an excised Ll.ltrB
intron RNA and the LtrA protein were prepared by transforming host cells as described above in example 1 except that the LtrA ORF was tagged at the N-terminus with a Hisb affinity tag and the epitope tag XPRESSTM which was obtained from Invitrogen, San Diego, CA. The tag is used to facilitate isolation of the RNP particles. The plasmid adding the tags was made in two steps by using PCR. In the first step, a fragment was made in two steps by using PCR
mutagenesis. In the first step, the LtrA ORF and 3' exon were amplified and BamHl sites were appended to both the 5' an 3' end of the LtrA ORF using pLEl2 as a substrate and the following pair: 5' primer N-LtrA 5', having the sequence 5'CAAAGGATCCGATGAAACCA ACAATGGCAA 3', SEQ. ID. NO. 9; and the 3' primer LtrAex2, SEQ. ID. NO. 8. The PCR product was cut with BamHl and the resulting restriction fragment was gel purified and cloned inta the BamHl site of plasmid pRSETB
obtained from Invitrogen, San Diego, CA. The resulting plasmid pIntermediate-N
fuses the N terminus of the LtrA ORF to a Hisb purification tag, and adds an XPRESSTM
epitope tag from the vector. In a second step, the 5' exon and LLItrB intron sequences 5' to the ORF
were amplified using pLEl2 as a substrate and the 5' primer NdeLTRS, having the sequence 5'AGTGGCTTCCATATGCTTGGTCATCACCTCATC 3', SEQ. ID. No. 10 and 3' primer NdeLTR3', which has the sequence 5' GGTAGAACCATATGAAATTCCTCCTCCCTAATCAATTTT 3', SEQ. ID. NO. I 1. The PCR product was cut with Nde I, the fragment gel purified and cloned into plntermediate-N, which had also been cut with Nde I. Plasmids were screened for the orientation of the insert, and those oriented such that the 5' exon was proximal to the T7 promoter were used to transform the host cells. The resulting plasmid pFinal-N expresses a message under the control of the T7 polymerase promoter which comprises the El and E2 portions of the exons 1 LtrBEI and LtrBE2, and the LtrA ORF fused at the 5'end with an Hisb purification tag and the XPRESST"'' epitope tag.
Cells of the BLR(DE3) strain of E. coli were transformed as described in example 1 with plntermediate-N and cultured at 37°C f or 3 hours in SOB medium as described in SUBSTITUTE SHEET (RULE 26) example 3. The cells were also fractionated into a soluble fraction, which contains RNP
particles having nucleotide integrase activity, and an insoluble fraction as described in example 1. The RNP particles were further purified as described in example 1.

RNP particles having nucleotide integrase activity and comprising an excised Ll.ltrB
intron RNA and the LtrA protein were prepared as described by transforming host cells as described above in example 1 except that the LtrA ORF was tagged at the C-terminus with an intein from Saccharomyces cerevisiae VMA 1 gene and the chitin binding domain (CBD) from Bacillus circulan.r . The tag was used to facilitate purification of the RNP particles and was added using components of the Impact="" purification system obtained from New England Biolabs, Beverly, MA. A plasmid adding the tags was made in two steps by using PCR. In the first step, the LtrA ORF was amplified by PCR using pETLtrA 19 as template and using 5' primer LtrAexpr, 5'-AAACCTCCATATGAAACCAACAATG-3', SEQ. ID.
NO. and 3' primer ltrimpact: 5'TAACTTCCCGGGCTTGTGTTTATGAATCAC-3', SEQ. ID. NO. which deletes the termination codon and introduces a SmaI site.
The PCR product was cut with NdeI and SmaI and cloned into pCYB2, obtained from New England Biolabs, Beverly, MA, and cleaved with the same enzymes. Colonies were screened for inserts and two independent colonies with the desired insert were retained to yield pLI 1 PInt21 and pLI 1 PInt22. In a second step, pLI 1 PInt21 was cleaved with PstI, the overhangs repaired with T4 DNA polymerase in the presence of 0.2 mM dNTPs. The DNA
was then phenol extracted, ethanol precipitated and then partially digested with Pml I. The approximately 1580 by PmII- Pst I fragment was cloned into pETLtrAl9 digested with Pml I.
The clones with correct insert were screened and one oriented such that the intein is fused to the C terminus of the LtrA ORF was called pLI llnt. The resulting construct expresses the Ll.ltrB intron and fuses the LtrA ORF with the sequences that encode VMAI
intein and CBD.
Cells of the BLR(DE3) strain of E. coli were transformed as described in example 1 with pLlInt. The transformants were restreaked on ampicillin selective plates and single colonies were inoculated inta 50 mL of LB medium and grown overnight at 37° C. This culture was used to inoculate 0.5 liters of SOB in 4 liter flasks at a 1:100 dilution. The cultures were grown to an OD5~5 0.7-1.0 and induced with 1mM IPTG at room temperature for 4 hours. The cultures were harvested, washed with 150 mM NaC 1 10mM Tris-HCl (pH

SUBSTITUTE SHEET (RULE 26) 7.5), and repelleted and stored in 50 ml of Buffer I (20 mM Tris-HC 1 (pH8.0), 0.5 M NaC 1, 0.1 mM EDTA, 0.1 % NP-40). The cells were broken by sonicating for I minute 3 times in a Bronson sonicator at setting 7. The lysate was cleared by centrifugation at 12,000 x g for 30 minutes. The cleared lysate was loaded on a chitin affinity column equilibrated with Buffer I.
The RNP particles comprising a tagged protein are retained on the column. Then 15 ml of elution buffer (Buffer I+30 mM DTT) was passed through the column, the column flow was stopped, and the column incubated overnight at 4° C to allow self cleavage of the intein tag and release of the purified RNP particles from the chitin. Flow was restarted and the RNP
particles comprising an excised LLItrB intron RNA and the LtrA protein were collected.

RNP particles having nucleotide integrase activity and comprising the LtrA
protein and an excised LLItrB intron RNA having an altered EBS1 sequence were prepared as described above in example 1 except that the cells were transformed and the RNP particles were made using pLI 1-EB S 1 /-6C. The pLI 1-EBS 1 /-6C construct which has a single nucleotide change G to C at position 6 in the EBS 1 (G3137C as based on Mills et al, 1996) sequence of the wild-type intron and a complementary change in the 5' exon at position -6 relative to the 5' splice site to permit splicing was constructed via two PCR
steps. In the first step pETLtrAl9 was subjected to PCR with primers OP2, 5'-GGATCGAGATCTCGATCCCG, SEQ. ID. NO. and IP11: 5'CGCACGT
TATCGATGTGTTCAC, SEQ. ID. NO. to introduce the single nucleotide change in the exon, and with primers IP4, S'-TTATGGTTGTCGACTTATCTGTTATC, SEQ.ID.NO.-and OPI, OP1: 5'-CTTCGAATACCGGTTCATAG, SEQ. ID. NO. to introduce the single nucleotide change in EBS 1. The single nucleotide change in the IP4 primer introduces a SaII site in the EBS 1 sequence, which was subsequently used to identify the desired clones.
The second PCR step was performed using the above two PCR products as Primers and pETLtrAl9 DNA linearized with BgIII and BamHI as the template. The second PCR
product was reamplified with flanking primers OP2 and OP 1 using Pfu polymerase from Stratagene and digested with BgIII and BsrGI to yield a 554-by fragment that was cloned between the BsrGI and BgIII sites of pETLtrAl9. The desired clones were identified by digestion with HindIII and SalI, and the region that had been generated by PCR was sequenced completely to insure that no adventitious mutations had been introduced.

SUBSTITUTE SHEET (RULE 26) A partially-purified preparation of the LtrA protein, which is encoded by the ORF of the Ll.ItrB intron, using plasmid pETLtrA 1-1 was prepared. Plasmid pETLtrA 1-1 is ~
derivative of pETLtrAl9 and lacks exon 1 and the intron sequences upstream of the LtrA
ORF. Accordingly, the LtrA ORF is directly downstream of the phage T7 promoter following the Shine-Dalgarno sequence in the plasmid. The plasmid map of pETLtrAI-1 is shown in Figure 5.
pETLtrAI-1 was made by using the polymerase chain reaction to amplify the LtrA
ORF using the 5' primer LtrAexpr . SEQ.ID. , which introduces an NdeI site and 3' primer LtrAex2, SEQ. ID. NO. 8. The PCR product was cut with NdeI and BamHI, gel purified on a 1%. agarose gel, and cloned into pET-l la. The inserts of pLEl2, pETLtrAl9 and pETLtrA 1-1, each of which contain the LtrA ORF are depicted in Figure 6.
pETLtrAI-1 was introduced into cells of the E. coli strain BLR(DE3) as described in Example 1 and the transformed cells grown for 3 hours in SOB medium at 37°C as described in Example 3. Thereafter, the cells were lysed and the resulting lysate fractionated into a soluble fraction and insoluble fraction by low speed centrifugation as described in Example 1 to provide fractions containing a partially-purified preparation of LtrA
protein.
Preparing Nucleotide Integrases using in vitro-synthesized intron RNA

RNP particles having nucleotide integrase activity and comprising an excised, Ll.ltrB
intron RNA which lacks the ORF and an LtrA protein was prepared by mixing an in vitro-synthesized intron RNA with an LtrA protein preparation that was made by digesting the RNP particles prepared as described above in example 1 with micrococcal nuclease (MN).
Specifically, 1.0 O.DZbo of the RNP particle preparation were resuspended in 40 pl of 10 mM
Tris, HCI, pH 7.5, 10 mM MgClz, 2.5 mM CaCI,, 5 mM DTT and incubated with 12 or 36 units of MN from Pharmacia for 10 minutes at 22° C , after which the MN
was inactivated by addition of EGTA to 7.5 mM.
The group II intron RNA was generated by in vitro transcription of pLI2-DORF.
pLI2-DORF, which has a large deletion in the intron ORF, was derived from pLI2 by inverse PCR with primers ~ORFa: 5'-GGGGGGGCTAGCACGCGTCGCCACGTAATAAATATCTG GACG, SEQ. ID.
NO. and DORFb: 5'-GGGGGGGCTAGCACGCGTTGGGAAATG GCAATG ATAGC, SEQ.ID.NO. , each containing an MIuI site. The PCR product was digested with MIuI and SUBSTITUTE SHEET (RULE 26) self ligated to generate pLI2-tlORF, thereby replacing amino acids 40 to 572 of the LtrA
ORF with threonine and arginine. The plasmid was linearized with BamHI and transcribe with phage T3 RNA polymerase, and the in vitro-synthesized RNA (30 to SO~g) was spliced for 60 min at 42°C in 100 pl of 1 M NH4C1, 100 mM MgClz, and 50 mM Tris-HC 1 (pH 7.5).
S Prior to reconstitution, the RNA was heated to 85 to 90°C for 2 minutes, then stored on ice.
0.05 O.D.zbo units of the MN-treated RNP particles was added to 20 pl of reaction medium containing 50 mM Tris-HCl (pH7.5), 10 mM MgCl2, 10 mM KCI, 5 mM DTT, and 1 p.g of the spliced RNA to provide RNP particles having nucleotide integrase activity and comprising a modified, excised, Ll.ltrB intron RNA and an LtrA protein.
EXAMPLE 11.
RNP particles having nucleotide integrase and comprising the LtrA protein and an excised Ll.ItrB intron RNA having a kanamycin resistance gene inserted in domain IV in place of the LtrA ORF were prepared as described above in example 10 except that the RNA
component was made using pLI2-~ORFkanR. pLI2-DORFkanR, which replaces amino acids 39-573 of the LtrA ORF with a kanR gene, was constructed by cloning the 1,252-by SaII
fragment containing the kanR gene from pUK4K (Pharmacia, Piscataway, NJ) into the MIuI
site of pLl2-ORF by blunt-end ligation after filling in both the SaII and MluI
sites with Klenow polymerise (Life Technologies, Gaithersburg, MD) Comparative Example A
RNP particles lacking nucleotide integrase activity were prepared as described in Example 1 from cells of the BLR(DE3) strain of E. coli that had been transformed with plasmid pETI la, which lacks a group II intron. Accordingly, is these RNP
particles do not comprise excised, group II RNA or group II intron-encoded proteins and therefore, do not have nucleotide integrase activity.
Comparative Example B.
RNP particles lacking nucleotide integrase activity were prepared as described in Example 1 from cells of the BLR(DE3) strain of E. coli that had been transformed with plasmid pETLtrAI9FS, which comprises the sequence of an LtrA ORF having a frame shift 372 base pairs downstream from the initiation colon of the LtrA ORF. frame.
Accordingly, the RNP particles contain a truncated LtrA protein, i.e_ an LtrA protein lacking the Zn domain and, therefore, do not have nucleotide integrase activity.

SUBSTITUTE SHEET (RULE 26) Characterization of the RNP~articles of Examples 1 and 2.
A portion of the RNP particle preparation of examples 1 and 2 and comparative examples A and B were subjected to SDS polyacrylamide gel electrophoresis.
Staining of the resulting gel with Coomassie Blue permitted visualization of the proteins in each of the fractions. A band of approximately 70 kDa, which corresponds to the predicted molecular weight of the LtrA protein was seen in the lanes containing aliquots of the RNP particles of Examples 1 and 2. This band was absent from the lanes containing the RNP
particles prepared from comparative examples A and B. On the basis of the staining intensity of the 70 kDa band, the quantity of LtrA protein in 10 ODzGO units of RNP particles was estimated to be approximately 3 pg. Thus, RNP particles containing the group II intron-encoded protein LtrA can be prepared by expression of the group II intron Ll.ltrB in a heterologous host cell.
The reverse transcriptase activities of the RNP particles of examples l and 2 and the RNP particles of comparative examples A and B were assayed by incubating each of the RNP
particle preparations with a poly(rA) template and oligo (dT,g) as a primer.
The RNP particles of examples 1 and 2 exhibited reverse transcriptase activity, while the RNP
particles of comparative examples A and B exhibited no reverse transcriptase activity.
Thus, the methods described in examples 1 and 2 are useful for preparing RNP particles that have reverse transcriptase activity. The reverse transcriptase activity that is present in nucleotide integrases allows incorporation of a cDNA molecule into the cleavage site of the double stranded DNA which is cut by the nucleotide integrase.
Characterizing the Distribution and Yield of the LtrA Protein A portion of the insoluble fraction and soluble fraction of the lysates from the cells transformed and cultured according to the methods described in examples l, 2, 3, 4 and 9 were subjected to SDS polyacrylamide gel electrophoresis. Following electrophoresis, the SDS gels were stained with Coomassie blue to compare the yield of the LtrA
protein and the distribution of the 70 kDa LtrA protein prepared by the methods of examples 1, 2, 3, 4 and 9.
As shown on the gel, more of the LtrA protein was found in the soluble fraction when the transformed BLR (DE3) cells were grown in SOB medium and shaken at 300 rpm than when the transformed BLR cells were grown in LB medium and shaken at 200 rpm. In addition, the total amount of LtrA protein produced by the transformed BLR cells, that is the amount of LtrA in both the soluble and insoluble fractions, increased when, as described in example 4, a SUBSTITUTE SHEET (RULE 26) plasmid comprising the Ll.ltrB intron and a plasmid comprising argU(dna~ gene were both introduced into the host cells, the LtrA protein which was expressed in cells transformed with a plasmid which lacks the 5' segment of the Ll.ltrB.intron, as described in example 9, was significantly more insoluble than the LtrA protein which was expressed in cells transformed with a plasmid that contained the 5'segment of the intron as well as the LtrAORF.
Characterization of the Group II Intron-Encoded Protein Prepared According to the Methods of Examples 5-and 6.
A portion of the insoluble fraction and soluble fractions of the lysates from the cells transformed and cultured according to the methods described in examples 5 and 6 and in comparative examples A and B were subjected to electrophoresis on duplicate SDS-polyacrylarnide gels. One of the gels was stained with Coomassie blue and the proteins on the duplicate were transferred to nitrocellulose paper by Western blotting. A
primary antibody to the HSV antigen and an alkaline phosphatase-labeled anti-mouse IgG
secondary antibody were used in an enzyme-linked immunoassay to identify proteins carrying the HSV
epitope or the XpressTM tag. The anti-HSV antibody and the anti-XpressT"' tag antibody bound to a protein having a molecular weight of approximately 70 kDa, which is close to the calculated molecular weight of the LtrA protein. The HSV tagged LtrA protein and the XpressTM tagged LtrA protein were found in the soluble and insoluble fractions from cells transformed with pIntermediateC and pIntermediateN but not in the soluble fractions and insoluble fractions of cells transformed with pET27b(+) and pRSETB. Thus, the methods of examples 5 and 6 are useful for preparing an RNP particle comprising a tagged group II
intron encoded protein. These assays also demonstrated that the amount of the tagged group II intron-encoded protein present in the soluble fraction, from which the RNP
particles are derived, increases when the transformed and induced cells are incubated at 22°C as compared to 37°C. In cells grown at 22°C, the yield of the tagged protein was 0.4 to 2 mg per 1 culture, which is 2 to 5% of the total protein, with about 30% being soluble and 40 to 90% of the soluble protein being recovered in RNP particles (0.3 to 3 ~g LtrA
protein/O.D.26°). In cells grown at 37°C, a high proportion of the protein was insoluble. However, a significant amount of the tagged LtrA protein that was found in the soluble fraction was present in RNP
particles.

SUBSTITUTE SHEET (RULE 26) Characterization of the Purity and Yield of the Protein in the RNP Particles Prepared According to the Method of Example 7 A portion of the RNP particle preparation of example 7 and comparative examples A
and B were subjected to SDS polyacrylamide gel electrophoresis, which was subsequently stained with Coomassie Blue. A band of approximately 70 kDa, which corresponds to the predicted molecular weight of the LtrA protein was seen in the lanes containing aliquots of the RNP particles of Example 7 and was absent from the lanes containing the RNP particles prepared from comparative examples A and B. On the basis of the Bradford protein assays of the column eluant, the quantity of LtrA protein in RNP particles in the eluant from the chitin column was estimated to be approximately 0.5 mg/liter of start culture. The LtrA protein in these RNP particles was approximately 95% pure. Accordingly, the method of claim 7 is highly preferred for making large amounts of highly purified RNP particles having nucleotide integrase activity.
Using the RNP Particles to Cleave Double-Stranded DNA and to Insert Nucleotide Sequences into the Cleavage Site.
Nucleotide integrases are useful for cleaving RNA substrate, single-stranded DNA
substrates and one or both strands of a double-stranded DNA substrate, catalyzing the attachment of the excised, group II intron RNA molecule to the RNA substrate, the single-stranded DNA substrate, and to the first strand, i.e. the strand that contains the IBSl and IBS2 sequence, of the double-stranded DNA substrate. Nucleotide integrases also catalyze the formation of a cDNA molecule on the second strand, i.e. the strand that is complementary to the first strand, of a cleaved double-stranded DNA substrate. Thus, the nucleotide integrases are useful analytical tools for determining the location of a defined sequence in a double-stranded DNA substrate. Moreover, the simultaneous insertion of the nucleic acid molecule into the first strand of DNA permits tagging of the cleavage site of the first strand with a radiolabeled molecule. In addition, the automatic attachment of an RNA
molecule onto one strand of the DNA substrate permits identification of the cleavage site through hybridization studies that use a probe that is complementary to the attached RNA molecule.
An attached RNA molecule that is tagged with a molecule such as biotin also enables the cleaved DNA to be affinity purified. Moreover, the cleavage of RNA molecules, single stranded DNA
molecules, and one or both strands of a double stranded DNA molecule and the concomitant SUBSTITUTE SHEET (RULE 26) insertion of a nucleotide sequence into the cleavage site permits incorporation of new genetic information or a genetic marker into the cleavage site, as well as disruption of the clea~sl gene. Thus, the nucleotide integrases are also useful for rendering the substrate DNA
nonfunctional or for changing the characteristics of the RNA and protein encoded by the substrate DNA.
While RNP particles having nucleotide integrase activity can be used to cleave nucleic acid substrates at a wide range of temperatures, good results are obtained at a reaction temperature from about 30°C to about 42°C, preferably from about 30° to about 37°C. A
suitable reaction medium contains a monovalent cation such as Na+ or K+, and a divalent canon, preferably a magnesium or manganese ion, more preferably a magnesium ion, at a concentration that is less than 100 mM and greater than I mM. Preferably the divalent canon is at a concentration of about 5 to about 20 mM. The preferred pH for the medium is from about 6.0-8.5, more preferably about 7.5-8Ø
Because of its reverse transcriptase activity, the LtrA protein, either in the form of an RNP particle which comprises the LtrA protein or as a free protein, i.e., a protein which is not bound to a group II intron RNA, is also useful for transcribing RNA molecules.
Cleavage of Double Stranded DNA Substrates A. Cleaving a Double-Stranded DNA Substrate with the RNP Particles of Example 0.025 O.D 26° of the RNP particles of Example 1 and comparative examples A and B
were incubated for 20 minutes with 150,000 cpm of each of a 5' and 3' end-labeled double-stranded DNA substrate that comprises the wild-type exon 1 and the wild-type exon 2 junction of the Itt~B gene. The sequence of the 129 base pair substrate, which comprises the 70 base pair exon 1 and exon 2 junction of the ItrB gene, plus sequences of the plasmid is depicted in Figure 7A and SEQ. ID. NO. 4. To verify cleavage, the products were isolated on a 6% polyacrylamide gel.
The substrate which is cleaved by the nucleotide integrase, which comprises the excised LLItrB intron RNA and the LtrA protein, is schematically depicted in Figure 8(a). In addition, the IBS 1 and IBS2 sequence of the substrate is shown in figure 8(b). As shown in Figure 8, the IBS1 and IBS2 sequences which are complementary to the EBS
sequences of the Lltr.B intron RNA are present in exon 1 of the ltrB gene. As depicted in Figure 8, the RNP particles prepared according to the method of example 1 cleaved the sense strand of the substrate at position 0, which is the exon 1 and exon 2 junction, and cleaved the antisense SUBSTITUTE SHEET (RULE 26) strand at +9. When the RNP particles prepared according to the method of example 1 were treated with either RNase A/T1 to degrade the RNA in the particles, or with proteinase K~o degrade the protein component of the particles prior to incubation of the particles with the substrate, no cleavage of the substrate was observed. These results indicate that both the RNA component and the protein component of the nucleotide integrase are needed to cleave both strands of the substrate DNA.
0.025 O.D.,~o units of the RNP particle preparation of example 1 were reacted with 125 fmoles ( 150,000 cpm) of the 129 base pair internally-labeled DNA
substrate for 20 minutes. To verify cleavage, the products were glyoxalated and analyzed in a 1% agarose gel.
A dark band of radiolabel of approximately 1.0 kb RNA and lighter bands of approximately 0.8, 1.1, 1.4, 1.5, 1.G, 1.9, 2.5, 3.2 were observed on the gel.
Pretreatment of the reaction products with RNase prior to separation on the agarose gel resulted in the complete disappearance of these bands. These results indicate that the Ll.ltrB
intron RNA
was attached to the DNA substrate during reaction of the substrate with the RNP particles of example 1. On the basis of the size of Ll.trB intron, it is believed that the band at 2.5 kb represents the integration of the full length group II intron RNA into the cleavage site of the sense strand. The presence of smaller radiolabeled products on the gel is believed to be due to degradation of the integrated intron RNA by RNases which may be present during purification. The finding that the RNA-DNA products withstand denaturation with glyoxal indicates a covalent linkage between the intron RNA and the DNA substrate.
B. Cleaving Double-Stranded DNA Substrates using Nucleotide Inte~rases Prepared by the Methods of Examples 8. 10. and 11.
0.025 ~O.D.zbo units of the RNP particle preparation of examples 10 and 11 were reacted with 125 fmoles ( 150,000 cpm) of the 129 base pair internally-labeled DNA substrate for 20 minutes. To verify cleavage, the products were glyoxalated and analyzed in a 1%
agarose gel. To verify that the RNA component of the nucleotide integrase had been partially or fully integrated into the cleavage site, sequences of the exon 1 DNA-intron RNA and exon 2 DNA junctions were analyzed by RT-PCR. The RNP particles prepared as described in examples 10 and 11 were able to efficiently cleave the double-stranded DNA
substrate and to either partially or fully integrate the intron RNA subunit of the nucleotide integrase into the cleavage site. Thus, RNP particles that comprise LtrA protein and an Ll.ltrB
intron RNA
which lacks an ORF sequence have complete nucleotide integrase activity.
Similarly RNP

SUBSTITUTE SHEET (RULE 26) particles that comprise an LtrA protein and an LItrB intron RNA in which the ORF has been replaced with a sequence encoding a different gene product also have complete nucleotide integrase activity 0.025 O.D.zGO units of the RNP particle preparations of example 8 were reacted with S I 25 fmoles ( 150,000 cpm) of the I 29 base pair internally-labeled double-stranded DNA
substrate which comprises the sequence depicted in Figure 7A for 20 minutes.
In addition, 0.025 O.D.zeo units of the RNP particle preparations of example 8 were reacted with 125 fmoles (150,000 cpm) of a 129 base pair internally-labeled double-stranded DNA
substrate which comprises a modified exon 1 and wild-type exon 2 of the LLItrB gene for 20 minutes.
The sequence of the first strand of the 129 base pair substrate, in which the nucleotide at position -6 relative to the putative cleavage site in the wild-type exon 1 is changed from a C
to a G is underlined in Figure 7B. The putative cleavage sites in the first ~tranc~ r,f rhP
substrates shown in Figure 7A and 7B are depicted by a vertical line. To verify cleavage, the products were glyoxalated and analyzed in a 1% agarose gel. Endonuclease assays were also I S conducted to confirm that cleavage occurred between nucleotides -1 an +1 in the first strand of the substrate and at position +9 in the second strand of the substrate, and also to confirm that a nucleic acid molecule had been inserted into the cleavage site. The RNP
particles prepared as described in example 8 were able to efficiently cleave the double-stranded DNA
substrate shown in Figure 7b and to either partially or fully integrate the intron RNA subunit of the RNP particles into the cleavage site. The EBS I sequence of the modified Ll.ItrB intron in the RNP particles prepared as described in example 8 is complementary to the IBSl sequence of the substrate shown in Figure 7b. The RNP particles prepared as described in example 8, however, were not able to efficiently cleave the substrate depicted in Figure 7a.
The EBS 1 sequence of the modified Ll.ItrB intron in the RNP particles prepared as described 2S in example 8 is not complementary to the IBS 1 sequence of the substrate shown in Figure 7a.
These results indicate that changing the EBS 1 sequence of a group II intron RNA alters the target site specificity of the nucleotide integrase that comprises the modified group II intron RNA.

SUBSTITUTE SHEET (RULE 26j

Claims (20)

What is Claimed is:
1. A method of preparing RNP particles having nucleotide integrase activity comprising the steps of:
(a) providing an isolated, excised, group II intron RNA;
(b) providing a group II intron-encoded protein; and (c) incubating the excised, group II intron RNA with the group II
intron-encoded protein to provide an RNP particle comprising the excised, group II intron RNA bound to the group II
intron-encoded protein.
2. The method of claim 1 wherein the group II intron-encoded protein of step (b) is obtained by a process comprising the following steps:
a) expressing a DNA molecule which comprises an open reading frame sequence that encodes said group II intron-encoded protein in a host cell to provide an RNP particle comprising said group II intron-encoded protein bound to an RNA molecule;
b) lysing said host cell to obtain said RNP particle; and c) removing said RNA molecule from said group II intron-encoded protein.
3. The method of claim 2 wherein the DNA molecule lacks an intron sequence upstream of said open reading frame sequence.
4. The method of claim 3 wherein said open reading frame sequence is operably linked to a promoter.
5. The method of claim 2 wherein said RNP particle is obtained from a soluble fraction of the lysed host cell.
6. The method of claim 2 wherein the DNA molecule further comprises a nucleotide sequence encoding a tag for facilitating isolation of the RNP particle.
7. The method of claim 6 wherein the nucleotide sequence which encodes the tag is at the 5' end or the 3' end of the open reading frame sequence.
8. The method of claim 2 wherein the RNA is removed from the group II intron-encoded protein by contacting the RNP particle with a nuclease.
9. The method of claim 1 further comprising the step of introducing the DNA
molecule into a heterologous host cell prior to step (a).
10. The method of claim 1 wherein the group II intron-encoded protein is provided by a process comprising the following steps a) expressing a DNA molecule which encodes a wild-type or a modifed group II
intron RNA into a host cell to provide an RNP particle comprising said group II
intron-encoded protein bound to an RNA molecule;
b) lysing said host cell to provide said RNP particle; and c) removing said RNA molecule from said group II intron-encoded protein.
11. The method of claim 10 wherein the DNA molecule encodes a splicing-defective group II intron RNA.
12. The method of claim 10 wherein the RNP particle is obtained from a soluble fraction of the lysed cell.
13. The method of claim 10 further comprising the step of introducing the DNA
molecule into a heterologous host cell prior to step (a).
14. The method of claim 1 wherein the isolated, excised, group II intron RNA
is a wild-type group II intron RNA.
15. The method of claim 1 wherein the isolated, excised, group II intron RNA
is a modified group II intron RNA.
16. The method of claim 15 wherein the modified group II intron RNA comprises a modification in the loop region of domain IV.
17. The method of claim 15 wherein the modified group II intron RNA has a modified EBS 1 sequence.
18. The method of claim 15 wherein the modified group II intron RNA has a modified EBS2 sequence.
19. The method of claim 1 wherein said isolated group II intron RNA comprises a first hybridizing sequence capable of hybridizing with a first intron RNA binding sequence on one strand of a DNA substrate and a second hybridizing sequence capable of hybridizing with a second intron RNA binding sequence on said one strand of the DNA substrate.
20. The method of claim 16 wherein said isolated group II intron RNA further comprises a delta nucleotide that is complementary to a delta prime nucleotide on said one strand of the substrate, said delta prime nucleotide being located at position +1 relative to a cleavage site on said one strand of said DNA substrate.
CA002291512A 1997-05-28 1998-05-27 Methods of making an rnp particle having nucleotide integrase activity Abandoned CA2291512A1 (en)

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US5092297P 1997-05-28 1997-05-28
PCT/US1998/010687 WO1998054353A1 (en) 1997-05-28 1998-05-27 Methods of making an rnp particle having nucleotide integrase activity
US60/050,922 2008-05-06

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US6358712B1 (en) 1999-01-05 2002-03-19 Trustee Of Boston University Ordered gene assembly
WO2001029059A1 (en) 1999-10-15 2001-04-26 The Ohio State University Research Foundation Methods for analyzing the insertion capabilities of modified group ii introns
WO2005123962A2 (en) * 2004-06-14 2005-12-29 The University Of Texas At Austin Gene targeting in eukaryotic cells by group ii intron ribonucleoprotein particles
GB0612301D0 (en) 2006-06-21 2006-08-02 Morvus Technology Ltd DNA molecules and methods

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