AU2124601A - Molecular genetic constructions of vaccine strains of pasteurellaceae - Google Patents

Description

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P/00/011 Regulation 3.2

AUSTRALIA

Patents Act 1990 COMPLETE SPECIFICATION FOR A DIVISIONAL PATENT

ORIGINAL

TO BE COMPLETED BY APPLICANT Name of Applicant: Actual Inventor(s): BIOTECHNOLOGY RESEARCH AND DEVELOPMENT CORPORATION OF PEORIA, ILLINOIS AND U.S. DEPARTMENT OF AGRICULTURE Robert E. Briggs and Fred M. Tatum Address for Service: CALLINAN LAWRIE, 711 High Street, Kew, Victoria 3101, Australia

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C C C. C Invention Title: MOLECULAR GENETIC CONSTRUCTION OF VACCINE STRAINS OF PASTEURELLACEAE The following statement is a full description of this invention, including the best method of performing it known to me:- 14/02/01,cfl 1867.speci.doc,l U. w 2 MOLECULAR GENETIC CONSTRUCTION OF VACCINE STRAINS OF PASTEURELLACEAE BACKGROUND OF THE INVENTION Pasteurella haemolytica, P. multocida, and Haemophilus somnus are members of the Family Pasteurellaceae. Each is involved in respiratory disease syndromes in domestic cattle. These organisms have proven difficult to genetically manipulate, and therefore the construction of live, attenuated vaccines has been hampered.

Live attenuated bacterial strains generally provide superior protection as compared to killed bacterial vaccines (bacterins). In general, live vaccines elicit a stronger cell mediated response in the host than do bacterins. The superior immunity provided by attenuated live organisms may be explained by their ability to induce expression of stress-proteins and, possibly, of certain toxins within the host. The immune response generated by live organisms can be directed against these abundant proteins and thereby provide better protection.

There is a need in the art for live, attenuated vaccines against respiratory disease syndrome in domestic cattle caused by the Pasteurellaceae. There is also a need for techniques and tools to facilitate the construction of such vaccines.

SUMMARY OF THE INVENTION The invention provides a replication-conditional plasmid.

The invention also provides a cell-free preparation of a plasmid which is purified from genomic DNA and which is replication-conditional.

The invention further provides Pasteurellaceae host cells which comprise a plasmid which is replication-conditional.

The invention still further provides methods for introducing DNA into H. somnus.

The invention provides methods for mutagenizing H. somnus.

The invention also provides H. somnus transformant strains.

The invention further provides H somnus mutant strains.

14/02/01,cfl 1867.speci.doc,2 The invention still further provides genetically engineered H somnus.

In another aspect the invention provides a method of introducing a DNA segment into a Pasteurellaceae genome.

In a further aspect the invention provides genetically modified Pasteurellaceae.

These and other aspects of the invention are provided by one or more embodiments described below.

Accordingly, in one embodiment a plasmid which is conditional for replication in H. somnus, P. multocida, and P. haemolytica is provided.

In another embodiment of the invention a cell-free preparation of plasmid DNA which is purified free of genomic DNA comprising a plasmid which is temperature-conditional for replication in H. somnus, P. multocida, and P.

haemolytica is provided.

In another embodiment of the invention a host cell of the family Pasteurellaceae is provided. The host cell comprises a plasmid which is replicationconditional in H. somnus, P. multocida, and P. haemolytica.

In yet another embodiment of the invention a method of introducing a DNA segment to a Pasteurellaceae genome comprising: administering to a S. Pasteurellaceae cell a recombinant construct comprising the DNA segment and a :20 plasmid which is temperature-conditional for replication in the Pasteurellaceae cell to form transformants; subjecting the transformants to a non-permissive temperature; screening the transformants for the presence of the DNA segment; and screening the transformants for the absence of the plasmid is provided.

Preferably the DNA segment is a transposable element or a mutant form of 25 the genomic DNA of the Pasteurellaceae. Further preferably the mutant form is a deletion or an insertion.

In a further preferred embodiment the plasmid comprises an origin of replication of an incompatibility group comprising In yet another embodiment a genetically modified Pasteurellaceae is provided which is made by the method of administering to a Pasteurellaceae cell a recombinant construct comprising the DNA segment and a plasmid which is temperature-conditional for replication in the Pasteurellaceae cell to form 14/02/01,cfl 1867.speci.doc,3 transformants; subjecting the transformants to a non-permissive temperature; screening the transformants for the presence of the DNA segment; and screening the transformants for the absence of the plasmid.

These and other embodiments of the invention provide the art with the means to construct desirable mutants and transformants of the economically important and previously intractable Pasteurellaceae family of pathogens.

DETAILED DESCRIPTION OF THE PREFERRED EMBODIMENTS In the generation of defined mutations in the Pasteurellaceae, it is desirable to introduce a segment of the genome carrying a defined mutation which has been made either in vitro or in another bacterium. Typically, the segment of the genome is introduced on a plasmid. In order to "transfer" the defined mutation from the incoming DNA to the genome, homologous recombination is required. A single recombination event will result in integration of the entire plasmid, which results in one wild-type and one mutant copy of the gene. A second recombination event is desirable, to delete the wild-type copy of the gene and the vector sequences. Since the occurrence of the desired double recombination is a rare event, occurring in only a fraction of the cells which receive the introduced DNA, increasing the number of cells which contain the S introduced DNA will increase the recovery of cells which are double recombinants.

The use of a plasmid which can replicate in the Pasteurellaceae increases the S:.i number of cells which have the introduced DNA. However, the presence of a plasmid in cells which may ultimately be used for vaccines is undesirable, as such plasmids often contain ecologically and medically undesirable drug- and toxin-resistance determinants.

25 The inventors have solved this problem by creating a plasmid which does not replicate under defined conditions, which is conditional for replication. Thus genomic DNA carrying a defined mutation introduced to cells via the plasmid can be present in many copies in many directly transformed and progeny cells, by growing the cells at the permissive temperature. This feature increases the absolute number of desired double recombinants obtained by increasing the starting population of cells carrying the DNA-segment. In addition, by switching to the non-permissive conditions high temperature), one can eliminate plasmids which are episomal. It is a 14/02/01,cfl 1867.specidoc,4 discovery of the present invention that placing such plasmid-bearing bacteria at a higher temperature which does not permit efficient plasmid replication, results in quick loss of the plasmid.

The conditionality of the replication of the plasmids of the present invention can be based on any selectable phenotype. For example, the plasmids might be unable to replicate in the presence of a particular agent, such as a drug or toxin. The plasmids might not be able to replicate in the presence or absence of certain metabolites or salts. Temperature-conditionality has been demonstrated for a mutant of pD70, but other conditionalities can be used, as well as other plasmids which replicate in the Pasteurellaceae. Particularly preferred are those plasmids of the same incompatibility group as The plasmids of the present invention can be purified according to any art recognized method from genomic DNA. Typical separations of plasmid from genomic DNA in a cell-free preparation are electrophoretic, chromatographic, density gradient sedimentation, alkaline lysis, etc. The plasmids can be introduced into bacterial host cells of the Pasteurellaceae by any means known in the art, including transformation, conjugation, liposome mediated gene transfer, particle bombardment, etc. Any Pasteurellaceae host can be used.

Plasmid mutations may be induced by any means known in the art. These 20 include in vitro or in vivo chemical mutagenesis, passage through a mutator strain, etc. Even spontaneous mutations can be used if one is willing to screen more extensively. Particularly preferred are deletions and insertions which are nonreverting. Such mutations are easily generated in vitro using restriction enzymes, for example. Conditional mutations are most likely missense mutations, but nonsense S. 25 mutations can also be used in the presence of a temperature-sensitive suppressor tRNA.

The temperature-conditional plasmids of the present invention can be administered to a Pasteurellaceae cell according to standard methods known in the art, including, Sbut not limited to electroporation, transformation, transfection, transduction. One can screen by genetic or physical methods to detect those cells which have received the plasmid DNA. Subsequently, one can screen among the plasmid recipients for those which have lost the plasmid and retained the DNA of interest carried on the plasmid.

14/02/01,cfl 1867.speci.doc,5 u 1 6 The screening methods can be genetic or physical, such as screening for a phenotype or screening for the presence of a particular DNA sequence in the cell by hybridization.

It is an additional discovery of the present invention that H. somnus contains a restriction-modification system, called herein the Hsol system. The Hsol restriction endonuclease has been isolated and its cleavage sequence determined to be GCGC-3'. It has also been discovered by the present inventors, that a barrier to transformation of H. somnus can be overcome by treating DNA with a methylating enzyme, such as the Hsol methyl transferase Hsol). Such enzymes modify DNA substrates such that endonucleases which recognize 5'-GCGC-3' sequences are inhibited in their ability to digest such modified substrates. The methyl transferases produce a site which is 5'-GmCGC-3', the 5' cytosine is methylated. Examples of such methyl transferases are Hsol methyl transferase, HinPI methyl transferase, and Hhal methyl transferase, which is commercially available from New England Biolabs, Beverly, MA, 01915. Cells containing such methyl transferase enzymes can also be used. Preferably, these are recombinant cells with the methyl transferase enzymes introduced, so that they lack the cognate restriction enzyme. Alternatively, they are mutant or natural variants which lack the cognate restriction enzyme. In some instances, it may be possible to passage DNA through cells which have both the 20 restriction and methyl transferase enzymes, if the former is less active (slower) or less prevalent than the latter.

Methylation of DNA substrates for transformation (electroporation, or other S* means of introduction of DNA into cells) can be accomplished in vitro or in vivo. For in vitro methylation, DNA is incubated with a preparation of methyl transferase in the 25 presence of a methyl donor, such as S-adenosylmethionine (SAM). In vivo methylation can be accomplished by passaging the DNA substrate through a bacterium which contains an appropriate methyl transferase, such as Hsol, HinPI, or Hhal methyl transferase. A mutant or natural variant of H. somnus which lacks the S° Hsol endonuclease could also be used to prepare DNA for subsequent introduction into H. somnus. Such a mutant can be made inter alia according to the method for site-directed mutagenesis disclosed herein.

Site-directed mutagenesis of H. somnus can be accomplished according to 14/02/01,cfl 1867.speci.doc,6 the present invention by first isolating a wild-type DNA region from H. somnus. A mutation is created in the isolated, wild-type DNA region according to any method known in the art. For example, the isolated DNA can be chemically mutagenized, either in a bacterium or in vitro. Alternatively, restriction endonucleases can be used to create precise deletions or insertions in vitro. Other methods as are known in the art can be used as is desirable for a particular application.

After H. somnus DNA has been isolated and mutagenized, it is methylated as described above. Then it can be introduced into H. somnus according to any technique known in the art, including but not limited to transfection, transformation, electroporation, and conjugation. Alternatively, rather than methylating the mutagenized DNA and introducing it into a H. somnus which expresses Hsol restriction endonuclease, one can omit the methylation of the mutagenized DNA and introduce the mutagenized DNA into an H. somnus, H. haemolyticus, or H. influenza cell which does not efficiently express the Hsol restriction endonuclease or an isoschizomer of it. Such cells can be isolated from nature by extensive screening, isolated following chemical mutagenesis of a cell which does express the Hsol restriction endonuclease, or made by the site-directed mutagenesis method disclosed herein. According to one aspect of the invention, the mutagenized and 2 methylated H. somnus DNA region is introduced into a P. multocida cell on a plasmid 20 which includes a P. haemolytica approximately 4.2 kb streptomycin resistance determining plasmid (pD70). This plasmid has also been deposited at the American Type Culture Collection, 12301 Parklawn Drive, Rockville, MD, 20852, USA, on December 2, 1993, under the terms of the Budapest Treaty as Accession No. ATCC 69499. Derivatives of this plasmid or other pD70-incompatible plasmids (ie. plasmids 25 of the same incompatibility) can be used similarly. An incompatibility group is a group of plasmids which are so similar that a second member of the group cannot be added to a cell containing a first member of the group. The origin of replication of pD70 can be isolated on a 1.2 kb Sau3Al fragment immediately downstream of the streptomycin resistance determinant. Gene conversion can be monitored inter alia by Southern hybridization with probes to the gene of interest, by screening for genetic markers on the introduced DNA construct (such as ampicillinR or streptomycinR), and by screening for the presence/absence of plasmid in the transformed cells' progeny.

14/02/01,cfl 1867.speci.doc,7 Also provided by the present invention are mutant and transformant strains made by the disclosed methods of transformation and/or site-directed mutagenesis.

Such mutants can provide the veterinary arts with attenuated, live strains of Pasteurellaceae, which are suitable for vaccines to induce protective immunity against Pasteurellaceae infection. For vaccine production, it is desirable that the mutation which attenuates the bacterium be an essentially non-reverting mutation.

Typically these are deletion or insertion mutations, the latter not being caused by a transposable element. Strains which contain multiple attenuating mutations may also be used, so that the risk of reversion to a wild-type, virulent bacterium is vanishingly small. Suitable attenuating mutants may be, for example, auxotrophic. Mutants with altered virulence factors may also be used.

One mutant strain which can be made by the site-directed mutagenesis method disclosed is one which is Hsol restriction endonuclease negative. Such a strain is useful for genetic engineering in H somnus. Such a strain can be a recipient of DNA which is not Hsol methyl transferase methylated, yet would yield DNA which is Hsol methyl transferase methylated.

A preparation of isolated Hsol endonuclease can be prepared inter alia by passing a cell-free lysate of H. somnus over a column of heparin-sepharose. Other known techniques for isolating restriction endonucleases can be used as is 20 appropriate.

Typically the specific activity of such a preparation will be enriched as compared to the cell-free lysate.

S* The present invention thus allows those of ordinary skill in the art to stably introduce DNA into H. somnus. The DNA can be from other strains or species. The S: 25 DNA can be artificially modified or in its native state. If recombination into the o* genome is desired two regions of flanking homology are preferred. Such techniques are generally known for other bacteria, but have been hitherto unsuccessful in H.

00 somnus due to its restriction system.

Vaccines are typically formulated using a sterile buffered salt solution.

Sucrose and/or gelatin may be used as stabilizers, as is known in the art. It is desirable that the Pasteurellaceae vaccines of the invention be administered by the intranasal or intratracheal route, but subcutaneous, intramuscular, intravenous 14/02/01,cfl 1867.speci.doc,8 9 injections also may be used. Suitable formulations and techniques are taught by Kucera U.S. 4,335,106, Gilmour U.S. 4,346,074, and Berget U.S. 4,957,739.

Typically, between 10 7 and 1011 CFU are administered per dose, although from 105 to 103 CFU can be used. Adjuvants also may be added.

EXAMPLES

Example 1: Plasmid construction and mutagenesis. The 4.2 kb plasmid which encodes streptomycin resistance in Pasteurella haemolytica serotype 1 has been previously sequenced and described (Chang, Tatum). The plasmid was linearized by Hindlll digestion and made blunt by treatment with dNTPs and Klenow fragment. A kanamycin cassette (Genblock) previously digested with BamHI and made blunt as above was ligated into pD70 to produce pD70kan. This plasmid was amplified in E. coil DH10B containing Phal methyltransferase on cosmid Phalmtase.

The plasmid was introduced into P. haemolytica strain NADC-D153. Plasmid DNA (1 pg) recovered from a kanamycin-resistant transformant was mutagenized with hydroxylamine for 90 minutes at 700 C as previously described. The treated DNA was dialyzed against TE, ethanol-precipitated, and resuspended in TE (10 mM Tris, 1 mM EDTA, pH 20 Example 2: Recovery of temperature-sensitive plasmids. Pasteurella haemolytica serotype 1, strain NADC D153, was grown to late logarithmic phase in 100 ml columbia broth at 370 C with gentle shaking. The bacteria were pelleted by S centrifugation at 5000 x G and washed in 100 ml 272 mM sucrose at 0° C. The pellet was resuspended in an equal volume of 272 mM sucrose at 00 C. Competent cells 25 (100pl) were placed into six 0.1 cm electroporation cuvettes and mixed with 100 ng of the treated DNA. The cells were electroporated (GenePulser, Bio-Rad) at 18,000 V/cm and 800 ohms yielding time constants ranging from 11-12 msec. Immediately after each electroporation the cells were resuspended in 1.0 ml columbia broth at 00

SC.

Recovery was for 2 hours at 300 C. The suspension was spread (100 pl plate) onto columbia agar (Difco) plates containing 50 pg/ ml kanamycin. Plates were incubated 28 hours at 30 0 C then transferred to 42° C for 6 hours. Colonies were 14/02/01,cfl 1867.speci.doc,9 picked which were smaller than typical colonies and dotted onto kanamycin plates.

After overnight incubation at 30* C, growth from each selected colony was duplicated onto columbia agar plates with and without kanamycin and then incubated overnight at 42 0 C. Growth from non-selective plates was transferred to kanamycin plates which were incubated overnight at 300 C. Clones which failed to grow with selection at 420 C but which grew well on selective media at 300 C after passage without selection at 420 C were presumed to be temperature-sensitive for kanamycin expression. Similar clones which exhibited reduced growth on selective plates at 300 C after passage without selection at 420 C were presumed to be temperature-sensitive for plasmid maintenance. Four of the latter clones were selected for further study.

Example 3: Testing of temperature-sensitive plasmids. Plasmid DNA was recovered by an alkaline lysis procedure from four P. haemolytica clones presumed to contain temperature-sensitive plasmid origins of replication. The DNA was electroporated into P. multocida strain NADC TT94, a bovine lung isolate which is Carter-Heddleston type A:3. After specific methylation with Hhal (as previously described) the DNA was electroporated into H. somnus strain HS91, a bovine lung isolate. Transformants were grown overnight on columbia agar plates supplemented S with 5% bovine blood and 50 pg/ml kanamycin at 300 C in 10% C00 2 Duplicate broth :20 cultures were inoculated with transformants of each organism and plasmid. One .i culture was grown overnight at 400 C, the other at 30 0 C. Plasmid was recovered from each broth by an alkaline lysis procedure and resolved on 1% agarose gels.

Selective and non-selective plates were struck for subjective assessment of percentage CFU resistant to kanamycm after passage.

Example 4: Properties of the replication-conditional plasmid. Pasteurella haemolytica was transformed to kanamycin resistance by the mutagenized plasmid at an efficiency of about 6x10 4 CFU/pg DNA. Of the transformants, about 1% (360) were found to form atypically small colonies after the incubation at 420 C. Passage of these colonies at either 300 C or 420 C on plates with or without kanamycin revealed that about 90% of the transformants were temperature sensitive for expression of kanamycin-resistance (about 10% failed to grow on the first passage and were not 14/0201,cfl I867.speci.doc,10

I

11 tested further). These organisms formed colonies on selective or non-selective plates at 30 0 C but failed to grow on selective plates at 42 0 C. Passage of growth from nonselective plates at 420 C to selective plates at 300 C resulted in heavy growth, indicating plasmid was still present. A 5.5 kb plasmid was detected in plasmid preparations out of representatives of these cultures.

Ten of the 360 colonies behaved on passage similar to the colonies containing temperature-sensitive kanamycin genes except growth was reduced on selective media at 300 C after passage without selection at 420 C. These colonies appeared to vary in percentage resistant to kanamycin after passage without selection at 42 0 C, indicating possible differences in their degree of instability at nonpermissive temperature (42 0 Four were selected based on their low yield of kanamycin resistant colonies after passage without selection at the non-permissive temperature.

The four temperature-sensitive plasmids were readily introduced into P.

multocida strain NADC-TT94 and into H. somnus strain NADC-HS91 (after appropriate methylation). The plasmids behaved as they did in P. haemolytica. No growth was observed on selective plates incubated at 400 C and no plasmid was detected in broth cultures grown without selection at 40° C. Cultures transformed with o wild-type plasmid grew well under selection at 400 C and yielded plasmid DNA from 20 non-selective broth cultures at that temperature. All cultures grew and yielded *9 plasmid when grown with or without selection at 30° C. The results indicate that plasmid replication is temperature-conditional in each of the three species bacteria.

°One of the temperature-conditional plasmids called pBB192 has been deposited in P. haemolytica NADC D153 at the American Type Culture Collection, 25 Rockville, MD, 20852 under Accession No. ATCC 55893 on December 2, 1996.

Example 5: Isolation and characterization of restriction endonuclease, Hsol, from Haemophilus somnus and protection of heterologous DNA by Hhal methyl goof*: transferase.

Chromatographic fractions exhibiting endonuclease activity eluted from the heparin-sepharose columns by 680 and 760 mm NaCI (960 1060 pS). A single pass through these columns was sufficient to identify both the recognition specificity and 14/02/01,cfl 1867.speci.doc,l I cleavage site. Digestion of lambda DNA with the concentrated Hsol preparation resulted in a distinctive restriction fragment pattern identical to that produced by Hhal, a commercially available restriction endonuclease isolated from Haemophilus haemolytica. The cleavage site was found to differ from that of Hhal, producing a 5' overhang identical to that produced by HinPI.

Methods Used Bacterium, growth, and crude extract. Haemophilus somnus, strain 2336 (kindly supplied by Lynette Corbeil, San Diego, CA), was grown for 16 h on eight chocolate agar plates (Columbia blood agar base; Difco, Detroit, Mich, supplemented with 5% defibrinated bovine blood at 90 0 C, 200-ml total volume). The cells were harvested in TE (10 mM Tris, 1 mM EDTA, pH pelleted by centrifugation at 16,000 x g for 5 min at 4 0 C, and washed once in TE. The washed pellet was resuspended in 12 ml chromatography running buffer (20 mM sodium phosphate, mM 2-mercaptoethanol, pH 8.0, 00 C) and placed on ice. The bacterial cells were disrupted by sonication for 2 mm in 15-s bursts. Debris and unbroken cells were removed by centrifugation at 16,000 x g for 10 min, and the supernatant was filtered 20 through a 0.45-pm-pore-size membrane (Millex-HA; Millipore Corp., Bedford, Mass.).

No further treatment of the crude extract was performed prior to chromatography.

Chromatographic separation of proteins. All chromatographic procedures were performed at room temperature. Prepacked heparin-Sepharose columns (Econopac 25 heparin columns; Bio-Rad, Richmond, Calif) were equilibrated as recommended by the manufacturer. A flow rate of 1.0 ml/min was used for separation, using a gradient low pressure automated chromatography system (Automated Econo-System; Bio- Rad, Richmond, Calif). Five ml of crude extract was injected and a linear gradient from 0 to 1.0 M NaC1 in 60 ml of running buffer was used to elute proteins. Fractions (1 ml) were stored on ice prior to activity assay. A second identical chromatographic separation was performed with a new column from which active fractions were collected and pooled for storage.

14/02/O1,cfl 1867.speci.doc,I 2 13 Assay for restriction endonuclease activity. Aliquots (5 pl) of the chromatographic fractions were incubated with 1 pl of React 1 (BRL, Gaithersburg, MD) and 0.5 pl of unmethylated bacteriophage lambda DNA (0.5 pg/pl; New England Biolabs, Beverly, Mass.) at 370 C for 2 h. After addition of tracking dye and electrophoresis on a 1% agarose gel in Tris-borate-EDTA buffer, the banding patterns were visualized by ethidium bromide staining and UV illumination. The fractions corresponding with DNA cleavage activity were pooled from the second chromatographic separation, concentrated 20-fold on 30,000-molecular-weight-cutoff ultrafilters, and brought to final concentrations of 150 mM NaCI, 10 mM sodium phosphate, 0.1 mM EDTA, 2-mercaptoethanol, 0.25 pg of bovine serum albumin per ml, and 50:50 (vol/vol) glycerol, pH 8.0, for storage at -20°C. The concentrated preparation was designated Hsol.

Determination of the recognition and cleavage sites for Hsol. The recognition sequence was identified by digestion of pBluescript (Stratagene, La Jolla, Calif.) and of lambda DNA. The cleavage site was identified by digestion of a primed-synthesis reaction on pBluescript. An oligonucleotide primer was synthesized which is complementary with sequences 3' from an Hsol site of pBluescript. Single-stranded 20 DNA was used for the template. Standard dideoxy DNA sequencing reactions were performed and an additional reaction containing no dideoxy terminator was extended through the Hsol site with the Klenow fragment of DNA polymerase I by using 32

P-

end-labeled primer. The extension reaction was stopped by phenol-chloroform extraction followed by ethanol precipitation. Hsol or Hhal (New England Biolabs) was 25 added to the additional reactions and allowed to digest the DNA for 2 min. The reaction was stopped by addition of gel loading buffer and heating to 800 C for 3 min.

S Example 6: Transformation of H. somnus with methylated DNA DNA obtained from Haemophilus somnus or from E. coli and in vitro methylated with Hhal methyl transferase was resistant to cleavage by both Hsol and Hhal. Protection by in vitro methylation was found to often be partial, based on electrophoretic mobility of DNA after digestion with and without prior in vitro methylation, even when the 14/02/01,cfl 1867.speci.doc, 3 4 14 substrate DNA had been phenol-chloroform-isoamyl alcohol extracted and then purified by CsCI gradient centrifugation.

Introduction of plasmid DNA into Haemophilus somnus was enhanced about 4 orders of magnitude by previous in vitro methylation of the plasmid. Each of the pD70-based plasmids transformed H. somnus, but efficiency dropped as the size increased. It is possible a second restriction-modification system may be responsible for the marked reduction in efficiency as plasmid size is increased. The possibility of systems analogous to mcr or mrr in E. coil was not investigated. Partial rather than complete protection conferred by in vitro methylation could also account for the reduction.

No ampicillin-resistant transformants were recovered, indicating either that the ampicillin-resistance cassette of pD80 does not express in H. somnus or that the origin of replication does not function. A pD70-based replicon containing the ampicillin-resistance cassette in the Hindlll site transformed H. somnus to yield streptomycin-resistant colonies. Those colonies failed to replicate on ampicillin containing media, indicating the ampicillin cassette does not function in H. somnus.

The pD80 origin of replication was not tested further.

kanamycin-resistance cassette derived from Tn903 was found to be excellent for selection of transformants. Streptomycin provided only fair selection.

20 Transformants containing both streptomycin- and kanamycin-resistance cassettes were more robust on kanamycin selection than on streptomycin. Conversely, untransformed colonies were common on streptomycin selection but were not encountered on kanamycin selection.

A second strain of H. somnus, 649 (kindly supplied by Dr. Lynette Corbeil), 25 was not transformed by derivatives of pD70. This strain was found to harbor a small plasmid which we presume to be incompatible with pD70. This plasmid, like might serve as a useful vector for the introduction of DNA into the bacterium.

The restriction-modification system carried by Haemophilus somnus are useful to genetically manipulate this pathogen. Specific methylation against the restriction endonuclease allows introduction of foreign DNA. Two replicons, both based on similar origins of replication, were discovered which may be of use as vectors for the introduction of foreign genes.

14/02/01,cfl 1867.speci.doc,14 Methods Used Construction and methylation of shuttle vector. A derivative of pD70, the 4.2 kb streptomycin-resistance plasmid of Pasteurella haemolytica serotype 1, was previously constructed during experiments involving that bacterium. Briefly, the 2.2 kb Pstl fragment of pD70 containing streptomycin-resistance was excised from a 1% agarose gel, electroeluted, and ligated with a Psti kanamycin cassette derived from Tn903 (Genblock, Pharmacia). The resulting plasmid conferred kanamycinresistance in E. coil and in P. haemolytica. The plasmid was methylated with commercially available Hhal methyl transferase according to instructions. Other plasmids based on the pD70 origin of replication were tested, including intact pD70kan (pD70 with the kanamycin cassette blunt-ligated into the unique Hindlll site), and pD80 (the 4.2 kb P. haemolytica plasmid encoding for ampicillinresistance).

Electroporation of methylated DNA into Haemophilus somnus.

20 Haemophilus somnus strain NADC Hs91 (pneumonic bovine lung isolate) was grown in Inn ml I v\inthnl'e hrnth at 37 0 in Ino/ Cntn I rt lo aririthmirc nh-ao ill iv uI l V VIIILII.U V I V.LI I ,L W I V. I v/ I U Z I. l .4ukr Iv U .I lU IIIII /I IC4W approximately four hours. The growth was pelleted by centrifugation at 5000 x G for fifteen minutes and washed once in 100 ml 272 mM sucrose at 00 C. The pellet was resuspended 1:3 packed bacteria 272 mM sucrose on ice. Competent bacteria (100 ml) were mixed with 100 ng plasmid DNA either unmethylated or in vitro methylated in 0.1 cm electroporation cuvettes (Bio-Rad). The cells were quickly electroporated after addition of DNA (Gene pulser, Bio-Rad) at 18,000 V/cm, 800 ohm, 25 mFd with resultant time constants ranging from 11 to 15 msec. Levinthal's broth (1 ml, 0°C) was immediately added to the electroporated cells and the suspension was incubated at 250 C approximately 10 minutes. The cells were then recovered at 370 C with 10% CO 2 for 2 hours. Ten-fold dilutions were plated onto chocolate agar plates (Columbia blood agar base with 5% defibrinated bovine blood) containing 50 mg ml 14/02/01,cfl 186 7 .speci.doc,l 16 kanamycin, 100 mg ml streptomycin, or 20 mg/ ml ampicillin. Colonies were enumerated after 36 hours incubation at 37 0 C with 10% CO 2 Representative colonies were examined for plasmid content using a rapid alkaline lysis procedure.

Example 7: Use of a temperature conditional replicon to generate an aroA deletion mutant of Pasteurella multocida Previous attempts to produce gene-replacement mutants of P. multocida in our lab were hindered by poor electroporation efficiencies and by replication of ColEIbased replicons in P. multocida (unpublished results). In addition, products of genereplacement typically contain foreign antibiotic resistance genes which may preclude or delay particular uses of otherwise desirable mutants. The shuttle plasmid constructed here was used to overcome those problems.

The origin of replication of the P. haemolytica plasmid pD70 was found to be within a 1.2 kb Sau3Al fragment downstream from the streptomycin coding region.

Together with a kanamycm cassette derived from Tn903, the vector (pBB192) proved to replicate in members of the Family Pasteurellaceae but not particularly well in E.

Scoli, requiring cloning of sequences relying on the pD70 origin to be performed in a Pasteurellaceae host. While unsuitable for use in P. multocida, a derivative of the shuttle vector was constructed which contains a ColE1 origin of replication in the 20 BamHI site (pBB192C) to facilitate construction in E. coli of temperature-conditional constructs for use in P. haemolytica or H. somnus target organisms (unpublished results). Plasmid pBB192C replicated efficiently in E. coli.

Approximately 100 P. multocida transformants were recovered on kanamycin at 30 0 C from electroporation with 25 ng of replacement plasmid. Passage of broth 25 cultures from 6 representative colonies to kanamycin plates at 40 0 C resulted in about well isolated colonies from each 10 pl inoculum, but the number of colonies produced varied among the 6 cultures. The colony size varied significantly on each plate, yielding a number of small colonies and a few large colonies. The relative proportion of these sizes varied among the 6 cultures. Southern blot analysis of genomic DNA from the colonies (probing with aroA) revealed that the small colonies were products of single crossover events. The large colonies contained sequences homologous to aroA which were not similar in size to the replacement plasmid in 14/02/01,cfl 1867.speci.doc,l 6 addition to a fragment consistent with wild-type chromosomal aroA. The large colonies were not examined further. Our interpretation of the data is that the integrated replacement plasmid destabilizes the chromosome, resulting in a substantial reduction in replication rate and therefore conferring small colony size.

The replacement plasmid, however, replicates so inefficiently by itself at the nonpermissive temperature that colonies do not form at all under kanamycin selection.

This situation put strong selective pressure to rearrange the plasmid for improved replication or to integrate into chromosome plasmid sequences containing the kanamycin gene, resulting in some potential unlikely products.

Passage of growth from products of single-crossover events without kanamycin selection resulted in >99% loss of kanamycin resistance in a single passage. These results indicate substantial instability of the single-crossover product.

Among 500 isolated colonies from such a passage, 5 failed to grow on both defined medium and under kanamycin selection. Southern blot analysis confirmed the loss of DNA sequences homologous to the deleted C/al EcoRV fragment, failed to show homology with plasmid vector, and showed a reduction of about 300 bp in size of chromosomal aroA. Results of PCR analysis indicated a 300 bp reduction in product size. Sequencing of the PCR product confirmed a deletion extending from the EcoRV site to slightly beyond the C/al site, 5'-ATTGATAT-GAACCAT-3', which does not alter 20 the reading frame of downstream DNA sequences.

The temperature-sensitive shuttle vector separated the operations of bacterial transformation from that of selection of crossover products in genereplacement. It also simplified the generation of products without foreign selectable markers. The instability of single-crossover products appeared to facilitate resolution S.i: 25 of the plasmid from the chromosome to generate deletion mutants without use of negative selection afforded by such genes as SacB. Since the vector replicates temperature-conditionally in P. haemolytica and in H. somnus, it is likely that it should S be equally useful in these or other Pasteurellaceae as well.

The P. multocida aroA mutant constructed here which was deposited on December 2, 1996, at the ATCC, and given the accession number ATCC 55892, differs from that described by Homchampa et al because the present strain is of bovine origin, a deletion was introduced in aroA, and no foreign DNA sequences are 14/02/01,cfl 1867.speci.doc,l7 present in the product. This mutant can be used as an attenuated live vaccine.

Methods Employed Construction temperature-sensitive shuttle vector. A shuttle-vector was constructed based on the previously described temperature-sensitive origin of replication of pD70, the streptomycin-resistance plasmid isolated originally from P.

haemolyica serotype 1 (Tatum et al, Chang). A PCR product approximately 1450 bp was produced from temperature-sensitive pD70kan #192 using forward primer GCCTGTTTTTCCTGCTC-3' and reverse primer The product was digested with Sau3Al to completion to produce an approximately 1.2 kb fragment. A kanamycin resistance cassette from Tn903 (GenBlock, Pharmacia) was digested with EcoRI, ligated into the EcoRI site of pBC SK (Stratagene), and electroporated into E. coli strain 30-9G to produce Phal-methylated plasmid DNA (Briggs et al). The approximately 1.3 kb kanamycin-resistance cassette was excised from the methylated plasmid with BamHI and ligated overnight to the 1.2 kb Sau3Al. The ligation mixture was electroporated into P. haemolytica strain NADC- D153 and plasmid was recovered from kanamycin resistant colonies. It was found that a portion of the pBC SK multiple cloning site from the EcoR1 site to the BamHI site had been transferred along with the kanamycin cassette, resulting in a 2.5 kb 20 plasmid with a unique EcoRI site and an effectively unique BamHI site which replicates in P. haemolytica, P. multocida, and H. somnus at 30 0 C but very poorly in E. coli. The plasmid was named pBB 192.

Cloning and Deletion of P. multocida aroA. A 1.2kb PCR product containing the 25 aroA gene was produced using forward primer TTACTCTCAATCCCATCAGCTATA-3' and reverse primer CTATCTGTAGGCTACTTCGCGTG-3'. The product was cloned into a vector which contains EcoR1 sites flanking the PCR product insert (TA vector, Invitrogen). The insert was excised with EcoR1 and ligated into the EcoR1 site of pUC9. The product was double digested with C/al and EcoRV to remove an approximately 300bp fragment. The ends of the remaining plasmid were made blunt using Klenow fragment of DNA polymerase I and dNTPs then ligated upon themselves to generate 14/02/01,cfl 1867.speci.doc,1 8 19 a deletion of aroA. The deleted plasmid was amplified in E.coli strain 30-9G to Phal methylate the DNA then digested with EcoR1 and electrophoresed on an agarose gel to confirm the deletion. The Phal-methylated EcoR1 aroA fragment containing the deletion was ligated into the EcoR1 site of pBB192 to create pBB 192PmAaroA. The ligation mixture was electroporated into P. haemolytica strain NADC-D153 and plasmid was recovered from kanamycin-resistant colonies.

Production of P. multocida single-crossover products. Pasteurella multocida strain NADC-TT94, a bovine lung isolate of Carter-Heddleston type A:3, was grown 4 hours in 100 ml columbia broth containing 2,500 U hyaluronidase. Growth was centrifuged at 5000 x G for 15 minutes and washed twice in 272 mM sucrose at 0° C then resuspended in 1 ml 272 mM sucrose. The cells (100 pl) were electroporated (Gene Pulser, Bio-Rad) with 25ng pBB192PmAaroA in a 0.1cm cuvette at 1.8kv, 8000, and 25 pF with a resultant time constant of 14.7 ms. The cells were immediately resuspended in 1 ml columbia broth at 0°C then incubated for 2 hours at 300 C. The recovered cells were spread 100 pl/plate on columbia agar plates containing 50 pg/ml kanamycin then incubated 24 h at 30°C. Six colonies were S* passed separately to 5 ml columbia broth containing 50pg/ml kanamycin which were incubated 18 hours at 300C. Growth was spread (10 pl plate) onto columbia agar plates with kanamycin which were incubated 24 hours at 40°C. Representative colonies were passed to columbia broth (25 ml) with kanamycin (to confirm single crossover products by Southern blot analysis) and to columbia broth (5 ml) without kanamycin (to screen for deletion mutants) and incubated overnight at 400C.

9 Screening for P. multocida deletion mutants. From the non-selective broth culture above, columbia agar plates were struck for isolated colonies and incubated overnight. Five-hundred isolated colonies were passed into microtiter plates containing 100pl columbia broth/well and incubated 6 hours. Growth (1 pl) was passed into each of two microtiter plates containing either 100pl/well columbia broth with kanamycin or 100 pl/well chemically defined medium lacking tryptophane based on that of Wessman et al 14/02/01,cfl 1 8 67.speci.doc, 9 v and that of Watko et al. Wells which grew only on the original non-selective microtiter plate but not on either kanamycin or defined medium were suspected deletion mutants. These were passed for Southern blot analysis and for PCR analysis using forward primer 5'-CTACCCACCTATCGCCATTC-3' and reverse primer TCCGCCCCCACCTTA-3'. The PCR product from one of the deletion mutants was cloned for sequencing of the deletion.

Where the terms "comprise", "comprises", "comprised" or "comprising" are used in this specification, they are to be interpreted as specifying the presence of the stated features, integers, steps or components referred to, but not to preclude the presence or addition of one or more other feature, integer, step, component or group thereof.

This is a divisional application of AU30596/97 the disclosure of which is incorporated herein by way of reference.

*o 14/02/01,cfl 1867.speci.doc,20

Claims (10)

1. A plasmid which is conditional for replication in H. somnus, P. multocida, and P. haemolytica.

2. The plasmid of claim 1 which comprises an origin of replication of an incompatibility group comprising pD70 (ATCC 69499).

3. The plasmid of claim 1 which comprises a pD70 origin of replication.

4. The plasmid of claim 1 which replicates at 30 0 C but fails to replicate at 42 0 C. The plasmid of claim 4 which has been deposited at the American Type Culture Collection as Accession No. ATCC 55893.

6. A cell-free preparation of plasmid DNA which is purified from genomic DNA comprising a plasmid which is temperature-conditional for replication in H.somnus, P.multocida, and P. haemolytica. 20

7. A host cell of the family Pasteurellaceae which comprises the plasmid of claim 1.

8. A host cell of the family Pasteurellaceae which comprises the plasmid 25 of claim 2.

9. A host cell of the family Pasteurellaceae which comprises the plasmid of claim 3.

10. A host cell of the family Pasteurellaceae which comprises the plasmid of claim 4. 14/02/01,cfl 1 8

67.speci.doc,21 I* V 11. of claim A host cell of the family Pasteurellaceae which comprises the plasmid 12. A method of introducing a DNA segment to a Pasteurellaceae genome comprising: administering to a Pasteurellaceae cell a recombinant construct comprising the DNA segment and a plasmid which is temperature-conditional for replication in the Pasteurellaceae cell to form transformants; subjecting the transformants to a non-permissive temperature; 0 screening the transformants for the presence of the DNA segment; and screening the transformants for the absence of the plasmid. 13. The method of claim 12, wherein the DNA segment is a transposable element. 9 oo 14. The method of claim 12, wherein the DNA segment is a mutant form of the genomic DNA of the Pasteurellaceae. 15. The method of claim 14, wherein the mutant form is a deletion. 16. The method of claim 14, wherein the mutant form is an insertion. 17. The method of claim 12, wherein the plasmid comprises an origin of replication of an incompatibility group comprising 18. A genetically modified Pasteurellaceae made by the method of claim 19. A genetically modified Pasteurellaceae made by the method of claim 13 A genetically modified Pasteurellaceae made by the method of claim 14/02/01,cfl 1867.speci.doc,22 I *is 23 21. A genetically modified Pasteurellaceae made by the method of claim 22. A genetically modified Pasteurellaceae made by the method of claim 16. 23. A genetically modified Pasteurellaceae made by the method of claim 17. 24. A plasmid which is conditional for replication in H. somnus, P. multocida, and P. haemolytica substantially as herein described with reference to the accompanying Examples. A cell-free preparation of plasmid DNA which is purified from genomic DNA comprising a plasmid which is temperature-conditional for replication in H.somnus, P.multocida, and P. haemolytica substantially as herein described with reference to the accompanying Examples. 26. A host cell of the family Pasteurellaceae which comprises the plasmid :i 20 of claim 1 substantially as herein described with reference to the accompanying Examples. 27. A host cell of the family Pasteurellaceae which comprises the plasmid of claim 2 substantially as herein described with reference to the accompanying 25 Examples. 28. A host cell of the family Pasteurellaceae which comprises the plasmid of claim 3 substantially as herein described with reference to the accompanying Examples. 14/02/01,cfl 1867.speci.doc,23 29. A host cell of the family Pasteurellaceae which comprises the plasmid of claim 4 substantially as herein described with reference to the accompanying Examples. 30. A host cell of the family Pasteurellaceae which comprises the plasmid of claim 5 substantially as herein described with reference to the accompanying Examples. 31. A method of introducing a DNA segment to a Pasteurellaceae genome comprising: administering to a Pasteurellaceae cell a recombinant construct comprising the DNA segment and a plasmid which is temperature-conditional for replication in the Pasteurellaceae cell to form transformants; subjecting the transformants to a non-permissive temperature; screening the transformants for the presence of the DNA segment; and screening the transformants for the absence of the plasmid substantially as herein described with reference to the accompanying Examples. .*o 32. A genetically modified Pasteurellaceae made by the method of claim 12 20 substantially as herein described with reference the accompanying Examples. 33. A genetically modified Pasteurellaceae made by the method of claim 13 S substantially as herein described with reference to the accompanying Examples. 25 34. A genetically modified Pasteurellaceae made by the method of claim 14 substantially as herein described with reference to the accompanying Examples. ,35. A genetically modified Pasteurellaceae made by the method of claim substantially as herein described with reference to the accompanying Examples. 36. A genetically modified Pasteurellaceae made by the method of claim 16 substantially as herein described with reference to the accompanying Examples. 14/02/01,cfl 1867.speci.doc,24 37. A genetically modified Pasteurellaceae made by the method of claim 17 substantially as herein described with reference to the accompanying Examples. Dated this 14 t day of February, 2000. BIOTECHNOLOGY RESEARCH AND DEVELOPMENT CORPORATION OF PEORIA, ILLINOIS AND U.S. DEPARTMENT OF AGRICULTURE By their patent attorneys CALLINAN LAWRIE *co eee.: 14/02/O1,cfl 1 8 67.speci.doc,25