COMPOSITIONS FOR USE AS A PROPHYLACTIC AGENT TO THOSE AT RISK OF INFECTION OF TUBERCULOSIS, OR AS SECONDARY AGENTS FOR TREATING INFECTED TUBERCULOSIS PATIENTS

Information

  • Patent Application
  • 20240382575
  • Publication Number
    20240382575
  • Date Filed
    July 30, 2024
    3 months ago
  • Date Published
    November 21, 2024
    5 days ago
Abstract
The present invention refers to a freeze-dried composition consisting of an isolated microorganism belonging to the Mycobacterium tuberucolosis complex, preferably a M. tuberculos clinical isolate, more preferably M. tuberculosis clinical isolate, characterized in that it comprises a PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype) (the MTBVAC strain), and sucrose and sodium glutamate as stabilizers or excipients. The present invention further refers to the reconstituted composition obtained by adding water, preferably sterilized water for injection, to the freeze-dried composition as well as uses thereof, in particular for use as a prophylactic agent to those at risk of infection with M. tuberulosis or those at risk of developing tuberculosis disease, or as secondary agents for treating infected tuberculosis patients.
Description
REFERENCE TO AN ELECTRONIC SEQUENCE LISTING

The contents of the electronic sequence listing (920201_401C2_SequenceListing.xml; Size: 9.67 kilobytes; and Date of Creation: Apr. 28, 2023) is herein incorporated by reference in its entirety.


FIELD OF THE INVENTION

This invention relates to pharmaceutical compositions, such as vaccines, and methods of making and using such compositions.


BACKGROUND OF THE INVENTION

Bacille Calmette-Guérin (BCG) vaccine is an attenuated strain of Mycobacterium bovis, the etiologic agent of tuberculosis (TB) in cattle. BCG was introduced for the first time into clinical use almost a hundred years ago, when in 1921 it was given orally to an infant whose mother had died of TB a day after delivery. The infant showed no adverse events to vaccination with BCG and importantly, did not develop TB. At that time, the oral route of BCG administration was considered the natural (gastrointestinal tract) route for acquiring TB in infants and children fed with unpasteurized milk. TB is poverty related with major burden in the poor and developing parts of the world. The incidence of TB is increasing worldwide due to poverty and inequity and is aggravated with the HIV/AIDS pandemic, which greatly increases risk of infection proceeding to active disease. Diabetes, metabolic syndrome, smoking and more recently vitamin deficiencies due to malnutrition and poor socioeconomic conditions are emerging as important risk factors for TB. Importantly, how these factors can influence efficacy evaluation of new TB vaccines requires specific attention when defining clinical trial designs that involve study or patient populations with a variety of such risk factors. Because of the rising globalization and emergence of multidrug-resistant (MDR) and extensively drug resistant TB (XDR) strains, TB is increasingly becoming a serious threat for the entire world.


Today TB has reached alarming proportions of 10.0 million incidence cases and 1.6 million deaths attributed to the disease as reported by the latest World Health Organization (WHO) global TB report 2018. Globally, some 50 million individuals are already latently infected with MDR M. tuberculosis strains creating a remarkable resource for future cases of active TB with insufficient treatment options. Nevertheless, the WHO End TB Strategy has vowed to reduce TB morbidity by 90% and TB mortality by 95% by 2035 and recognizes the urgent need for more accessible diagnostic tools that are rapid and reliable, new less toxic and more efficacious antibiotics to shorten therapy and ultimately new vaccines to prevent pulmonary TB in order to achieve this ambitious goal.


The present invention contributes to the objective of providing new vaccines to prevent TB.


BRIEF DESCRIPTION OF THE INVENTION

The present invention refers to a live-attenuated M. tuberculosis vaccine composition, preferably a reconstituted composition after freeze-drying, comprising an isolated microorganism belonging to a MTBVAC strain having a i) PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and ii) the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype), wherein said composition is characterized in that it comprises the following components per mL (in terms of percentages):
















MTBVAC



Components
Dose per 1 mL








L-Asparagine
0.034-0.066%



Monopotassium phosphate
0.006-0.010%



Magnesium sulfate H2O
0.008-0.012%



Ammonium ferric citrate
0.0004-0.0008%



Dextrose monohydrate
 0.05-0.066%



Glycerol
0.00005-0.0001% 



Citric acid
0.026-0.034%



Polysorbate 80
0.000002-0.000008%



Sodium glutamate
0.33-1.33%



Sucrose
 3.3-13.3%



Purified water QS
1 mL












BRIEF DESCRIPTION OF THE FIGURES

Other objects, advantages and novel features of the present invention will become apparent from the following detailed description of the invention when considered in conjunction with the accompanying drawings.



FIG. 1. Growth of the SO2 strain in Middlebrook 7H9 medium and synthetic Sauton medium. Results of OD and Cfu/mL of culture passes 1 and 2.



FIG. 2 shows the OD results of the MTBVAC cultures in Sauton, SD and SDG media.



FIG. 3 shows the stability results between 2-8° C. and −30° C. of the lots or batches identified in table 15.



FIG. 4 Protection in mice. Data in the figure represent a pool of two independent experiments (n=12 mice/group). All data are mean±SEM. Protection index is defined as the difference between bacterial load in unvaccinated and vaccinated groups (represented in decimal logarithm).



FIGS. 5A-5C. Immunogenicity in mice. Data in the figure are from one experiment (n=5 mice/group). All data are mean±SEM. SFC: Spot Forming Colony.



FIG. 6. Vaccination of neonates from a TB endemic setting with escalating doses of MTBVAC resulted in predominantly Th1 (IFN-γ, IL-2, or TNF-α) antigen-specific CD4 T-cell responses. The highest MTBVAC dose of 2.5×105 CFU induced the greatest magnitude of antigen-specific CD4 T-cells cytokine response at day 70. The lowest MTBVAC dose of 2.5×103 CFU was the least immunogenic.



FIG. 7. Vaccination of neonates from a TB endemic setting with escalating doses of MTBVAC resulted in a dose-response profile of the quantitative value of the QFT assay at day 180 and 360 post-vaccination. The QFT values are stratified in three different regions according to the risk of developing active TB as per Andrews JR, Nemes E, Tameris M et al. Serial QuantiFERON testing and tuberculosis disease risk among young children: an observational cohort study. Lancet Respir Med, (2017).



FIGS. 8A-8B. Absence of virulent mycobacteria in the working seed lot in Guinea pigs.



FIG. 9. Stability studies in the Master and working seed lots.



FIGS. 10A-10B. Long term stability study of MTBVAC vaccine 3-17×103 cfu/0.1 mL dose, 3-17×104 cfu/0.1 mL dose and 3-17×106 cfu/0.1 mL dose stored at −15° C.-−30° C., (A), and stored at +2° C.-+8° C., (B).



FIG. 11. Step-by-step construction from SO2 to MTBVAC. The final double-deletion strain is phenotypically identical to prototype SO2 (phoP−based PDIM− deficient) but provides greater assurance of genetic stability. Light blue depicts the phoP gene, fadD26 gene is shown in light orange, antibiotic resistance cassettes kmr and hygr are in magenta, yellow triangles depict res sites flanking Ωhygr or the residual res site in the deleted regions; res sites do not contain any exogenous coding sequence.





DETAILED DESCRIPTION OF THE INVENTION
Definitions and Detailed Description of the MTBVAC Strain

The “MTBVAC strain” will be used to refer to the isolated microorganism of the M. tuberculosis strain that has deleted the Rv0757 gene in M. tuberculosis MT103 clinical strain and which additionally comprises the deletion of the Rv2930 (fadD26) gene. Therefore, said strain presents two independent mutations derived from M. tuberculosis, the independent phoP deletion not affecting the properties of the vaccine derived from the inactivation of said gene. Therefore, “the MTBVAC strain” is characterized in that PDIM production is inactivated through the deletion of the Rv2930 (fadD26) gene, and thus this strain is characterized in that it comprises the deletion of the Rv2930 and Rv0757 genes.


It is thus noted that the MTBVAC strain was constructed to contain two independent non-reverting deletion mutations, without antibiotic markers, fulfilling the first Geneva consensus safety requirements for advancing live mycobacterial vaccines to phase I clinical evaluation. The MTBVAC strain was genetically engineered to phenotypically and functionally resemble its prototype SO2. SO2 is a marked Mt103 phoP mutant by the insertion of a kanamycin resistance cassette (kmr) (Mt103phoP::kmr) (see FIG. 11), which in addition to the engineered PhoP− deficient phenotype, SO2 has an acquired spontaneous loss in PDIM biosynthesis (see FIG. 2 of Dessislava Marinova, Jesus Gonzalo-Asensio, Nacho Aguilo & Carlos Martin (2017) MTBVAC from discovery to clinical trials in tuberculosis-endemic countries, Expert Review of Vaccines, 16:6, 565-576, DOI: 10.1080/14760584.2017.1324303), a process described to be common in M. tuberculosis as result of repeated laboratory subculture and manipulation practices.


As reflected in FIG. 11, MTBVAC strain was constructed following a stepwise approach. First, the unmarked deletion in fadD26 was introduced in SO2, giving rise to SO2ΔfadD26. Consequently, the unmarked deletion in phoP in SO2ΔfadD26 generated the MTBVAC strain. For construction of MTBVAC, suicide plasmids harbouring the deleted fadD26 and phoP genes, whose deleted regions were interrupted with a hygromycin resistance marker (hygr) flanked by res sites on each side (res::hygr::res), were used. γδ-resolvase from E. coli catalyzed the excision of the antibiotic resistance cassette following recognition of the res sites, thereafter leaving a copy of a residual res “scar” in place of the deletion (Malaga, et al. 2003); res sites do not contain any exogenous coding sequence. The final construct SO2ΔfadD26::ΔphoP was named MTBVAC strain. In the MTBVAC strain, the introduction of an unmarked deletion in fadD26 ensures a genetically stable abolishment of PDIM biosynthesis. The size of the generated deletion in the gene fadD26 comprises 1,511 bp and results in complete inactivation of this essential gene in PDIM biosynthesis. The wild-type gene is 1,752 bp (583 amino acids). A residual res scar was left in the process of the excision of hygr by γδ-resolvase. As a result of this deletion, the transcription levels of the next five genes in the PDIM locus (fadD26−ppsE) are diminished and PDIM biosynthesis in MTBVAC is completely abolished (Ainhoa Arbués PHD Thesis). The PDIM locus in M. tuberculosis comprises 13 genes clustered on a 50-kb fragment of the chromosome. The region is the biggest operon in the genome of M. tuberculosis (Camacho, et al. 2001; Camacho, et al. 1999; Cox, et al. 1999; Trivedi, et al. 2005).


In M. tuberculosis, phoP (744 bp) maps upstream of phoR (1458 bp) and both genes are transcribed in the same direction. Replacement of the generated 94-bp deletion within the phoP gene by the residual res site entails the presence of multiple STOP codons that on the other hand results in lack of translation of the DNA binding domain (equivalent to 92 amino acids) of PhoP in MTBVAC.


The deletions in phoP and fadD26 genes in MTBVAC can be detected/localised using a RT-PCR presence/absence approach. The method uses fluorescent-based PCR reagents (primers and probes) to indicate the presence of the res sites in ΔphoP and ΔfadD26 genes and absence of the wild-type phoP and fadD26 genes.


Herein below, we provide the open-reading frame (ORF) sequence of fadD26 gene in Mt103 a) and in MTBVAC (ΔfadD26) b); and the ORF sequence of phoP gene in Mt103 c) and in MTBVAC (ΔphoP) d). The nucleotide secquence corresponding to the deleted gene regions in fadD26 (a) and phoP (c) are depicted in small letters; residual res site is highlighted in grey. For the fluorescent-based PCR detection method, primers for each target are underlined and the Taq-man probe is shown in bold.









a) wild-type fadD26 gene in Mt103


SEQ ID NO 1


ATGCCGGTGACCGACCGTTCAGTGCCCTCTTTGCTGCAAG


AGAGGGCCGACCAGCAGCCTGACAGCACTGCATATACGTA


CATCGACTACGGATCCgaccccaagggatttgctgacagc


ttgacttggtcgcaggtctacagtcgtgcatgcatcattg


ctgaagaactcaagttatgcgggttacccggagatcgagt


ggcggttttagcgccacaaggactggaatatgtccttgca



ttcctgggcgcacttcaggctggatttatcgcggttccgc



tgtcaactccacagtatggcattcacgatgaccgcgtttc


tgcggtgttgcaggattccaagccggtagccattctcacg


acttcgtccgtggtaggcgatgtaacgaaatacgcagcca


gccacgacgggcagcctgccccggtcgtagttgaggttga


tctgcttgatttggactcgccgcgacagatgccggctttc


tctcgtcagcacaccggggcggcttatctccaatacacgt


ccggatcgacgcgtacgccggccggagtcattgtgtcgca


cacgaatgtcattgccaatgtgacacaaagtatgtacggc


tatttcggcgatcccgcaaagattccgaccgggactgtgg


tgtcgtggctgcctttgtatcacgatatgggcctgattct


cggaatttgcgcaccgctggtggcccgacgccgcgcgatg


ttgatgagcccaatgtcatttttgcgccgtccggcccgct


ggatcgacctgcgcgacgtggtcggcatcgtcagtggcag


tgagcgaatccatgtggcaaccgtgcggcggttcatcgag


cggttcgcgccgtacaatctcagccccaccgcgatacggc


cgtcgtacgggctcgcggaagcgaccttatatgtggcagc


tcccgaagccggcgccgcgcccaagacggtccgttttgac


tacgagcagctgaccgccgggcaggctcggccctgcggaa


ccgatgggtcggtcggcaccgaactgatcagctacggctc


ccccgacccatcgtctgtgogaatcgtcaaccoggagacc


atggttgagaatccgcctggagtggtcggtgagatctggg


tgcatggcgaccacgtgactatggggtattggcagaagcc


gaagcagaccgogcaggtcttcgacgccaagctggtcgat


cccgcgccggcagccccggaggggccgtggctgcgcaccg


gcgacctgggcgtcatttccgatggtgagctgttcatcat


gggccgcatcaaagacctgctcatcgtggacgggcgcaac


cactaccccgacgacatcgaggcaacgatccaggagatca


ccggtggacgggccgcggcgatcgcagtgcccgacgacat


caccgaacaactggtggcgatcatcgaattcaagcgacgc


ggtagtaccgccgaagaggtcatgctcaagctccgctcgg


tgaagcgtgaggtcacctccgcGATATCGAAGTCACACAG


CCTGCGGGTGGCCGATCTCGTTCTGGTGTCACCTGGTTCG


ATTCCCATCACCACCAGCGGCAAGATCCGGCGGTCAGCCT


GCGTCGAACGCTATCGCAGCGACGGCTTCAAGCGGCTGGA


CGTAGCCGTATGA.





b) ΔfadD26 in MTBVAC


SEQ ID NO 2


ATGCCGGTGACCGACCGTTCAGTGCCCTCTTTGCTGCAAG


AGAGGGCCGACCAGCAGCCTGACAGCACTGCATATACGTA


CATCGACTACGGATCCACTAGTTCTAGAGCAACCGTCCGA



AATATTATAAATTATCGCACACATAAAAACAGTGCTGTTA



ATGTGTCTATTAAATCGATTTTTTGTTATAACAGACACTG


CTTGTCCGATATTTGATTTAGGATACATTTTTATGAGATC


CCCCGGGCTGCAGGAATTCGATATCGAAGTCACACAGCCT


GCGGGTGGCCGATCTCGTTCTGGTGTCACCTGGTTCGATT


CCCATCACCACCAGCGGCAAGATCCGGCGGTCAGCCTGCG


TCGAACGCTATCGCAGCGACGGCTTCAAGCGGCTGGACGT


AGCCGTATGA.





c) wild-type phoP gene in Mt103


SEQ ID NO 3


ATGCGGAAAGGGGTTGATCTCGTGACGGCGGGAACCCCAG


GCGAAAACACCACACCGGAGGCTCGTGTCCTCGTGGTCGA


TGATGAGGCCAACATCGTTGAACTGCTGTCGGTGAGCCTC


AAGTTCCAGGGCTTTGAAGTCTACACCGCGACCAACGGGG


CACAGGCGCTGGATCGGGCCCGGGAAACCCGGCCGGACGC


GGTGATCCTCGATGTGATGATGCCCGGGATGGACGGCTTT


GGGGTGCTGCGCCGGCTGCGCGCCGACGGCATCGATGCCC


CGGCGTTGTTCCTGACGGCCCGTGACTCGCTACAGGACAA


GATCGCGGGTCTGACCCTGGGTGGTGACGACTATGTGACA


AAGCCCTTCAGTTTGGAGGAGGTCGTGGCCAGGCTGCGGG


TCATCCTGCGACGCGCGGGCAAGGGCAACAAGGAACCACG


TAATGTTCGACTGACGTTCGCCGATatcgagctcgacgag


gagacccacgaagtgtggaaggcgggccaaccggtgtcgc



tgtcgcccaccgaattcaccctgctgcgctatttcgtGAT



CAACGCGGGCACCGTGCTGAGCAAGCCTAAGATTCTCGAC


CACGTTTGGCGCTACGACTTCGGTGGTGATGTCAACGTCG


TCGAGTCCTACGTGTCGTATCTGCGCCGCAAGATCGACAC


TGGGGAGAAGCGGCTGCTGCACACGCTGCGCGGGGTGGGC


TACGTACTGCGGGAGCCTCGATGA.





d) ΔphoP in MTBVAC


SEQ ID NO 4


ATGCGGAAAGGGGTTGATCTCGTGACGGCGGGAACCCCAG


GCGAAAACACCACACCGGAGGCTCGTGTCCTCGTGGTCGA


TGATGAGGCCAACATCGTTGAACTGCTGTCGGTGAGCCTC


AAGTTCCAGGGCTTTGAAGTCTACACCGCGACCAACGGGG


CACAGGCGCTGGATCGGGCCCGGGAAACCCGGCCGGACGC


GGTGATCCTCGATGTGATGATGCCCGGGATGGACGGCTTT


GGGGTGCTGCGCCGGCTGCGCGCCGACGGCATCGATGCCC


CGGCGTTGTTCCTGACGGCCCGTGACTCGCTACAGGACAA


GATCGCGGGTCTGACCCTGGGTGGTGACGACTATGTGACA


AAGCCCTTCAGTTTGGAGGAGGTCGTGGCCAGGCTGCGGG


TCATCCTGCGACGCGCGGGCAAGGGCAACAAGGAACCACG



TAATGTTCGACTGACGTTCGCCGATATCGAATTCCTGCAG




CCCGGGGGATCTCATAAAAATGTATCCTAAATCAAATATC



GGACAAGCAGTGTCTGTTATAACAAAAAATCGATTTAATA


GACACATTAACAGCACTGTTTTTATGTGTGCGATAATTTA


TAATATTTCGGACGGTTGCTCTAGAACTAGTGGATCAACG


CGGGCACCGTGCTGAGCAAGCCTAAGATTCTCGACCACGT


TTGGCGCTACGACTTCGGTGGTGATGTCAACGTCGTCGAG


TCCTACGTGTCGTATCTGCGCCGCAAGATCGACACTGGGG


AGAAGCGGCTGCTGCACACGCTGCGCGGGGTGGGCTACGT


ACTGCGGGAGCCTCGATGA.






SO2 has a thorough and complete preclinical history demonstrating robust safety and attenuation profile and promising efficacy compared to BCG in relevant animal models. Fortunately, most of these preclinical studies have been reproduced with MTBVAC to confirm functional profile and biological activity of the double attenuating PhoP− PDIM− phenotype. Lipid profile analyses have demonstrated that MTBVAC and its prototype SO2 are phenotypically comparable lacking DAT, PAT, and PDIM.


On the other hand, from hereinafter in the context of the present invention, BCG will be used to refer to the current vaccine that has been in use against tuberculosis since 1921. It is a live attenuated vaccine derived from a M. bovis strain that lost its virulence after being sub-cultured in the laboratory and which we now know has more than one hundred deleted genes. Behr, M. A. BCG—different strains, different vaccines Lancet Infect Dis 2002, 2(2), 86-92.


From hereinafter in the context of the present invention, H37Rv will be used to refer to a pathogenic M. tuberculosis strain that has been sequenced, Cole et al. referring to these genes as Rv (Ref Cole et al 1998 Deciphering the biology of M. tuberculosis from the complete genome sequence. Nature 393: 537-544).


From hereinafter in the context of the present invention MT103 will be used to refer to a M. tuberculosis clinical isolate. Camacho et al. 1999 Identification of a virulence gene cluster of M. tuberculosis by signature-tagged transposon mutagenesis. Mol Microbiol 34: 257-267.


From hereinafter in the context of the present invention PDIM− strain will be used to refer to the strain of the M. tuberculosis complex that is not capable of synthesizing phthiocerol dimycocerosates, which are important lipids related to the pathogenicity of M. tuberculosis.


From hereinafter in the context of the present invention SO2+pSO5 will be used to refer to the M. tuberculosis SO2 strain in which the mutation in Rv0757 is complemented by the Rv0757 gene by transformation of a replicative plasmid with the mycobacterial phoP gene, but it is not capable of complementing PDIM synthesis, its phenotype being PhoP+ PDIM−.


From hereinafter in the context of the present invention M. tuberculosis phoP− will be used to refer to the M. tuberculosis strain that has been inactivated by the Rv0757 gene deletion between the EcoRV-BspEI sites, its phenotype being phoP− PDIM+.


From hereinafter in the context of the present invention Rv2930 (fadD26) will be used to refer to the gene that is at the beginning of the operon that is responsible for the synthesis of phthiocerol dimycocerosates (PDIM) (Camacho et al.) and the elimination of this gene in M. tuberculosis confers a stable PDIM− phenotype.


Description

The use of vaccines to prevent TB in humans has proven to be a tremendous challenge for almost a century now. BCG, derived from M. bovis, is currently the only licensed TB vaccine in use and is the most widely used vaccine in the world. The development and generalized administration of the BCG vaccine since the beginning of the 1920s represented a significant advance, with the prospect of being able to eradicate TB from the world. However, these initial promises were not achieved and, from the results of a large number of efficacy trials, it is clear that the BCG vaccine in its current form is of limited use in controlling the disease, particularly in respiratory forms in adults in third world areas where the disease is endemic. Fine, P.E. Variation in protection by BCG: implications of and for heterologous immunity. Lancet 1995, 346(8986), 1339-1345. With more knowledge of the virulence of M. tuberculosis and immune response models that lead to the generation of protective immunity, it is possible to develop better vaccines than BCG. The observation that higher protection levels are achieved when the host is vaccinated with BCG suggests that viability and persistence are fundamental properties required for the success of a tuberculosis vaccine. In this sense, in U.S. Pat. No. 8,287,886 B2 it was taught that the use a M. tuberculosis strain with the inactivated Rv0757 (phoP) gene and a second independent mutation of phoP, which prevents PDIM synthesis, provided for a prototype single dose live vaccine, which was more attenuated than BCG in immunocompromised SCID mice, provided protection levels comparable to those conferred by BCG in mice and higher protection than BCG in guinea pigs.


The phoP gene, together with phoR, forms part of a two-component system that shows a high degree of similarity to other two-component systems that control the transcription of key virulence genes in intracellular pathogens. It also controls the expression of many other genes that are not directly involved in virulence. Groisman, E. A. The pleiotropic two-component regulatory system PhoP−PhoQ. J Bacteriol 2001, 183(6), 1835-1842. The elimination of virulence genes does not seem to be, per se, the only method for the attenuation of M. tuberculosis. It was shown that a pantothenate auxotrophic mutant of M. tuberculosis, which is incapable of de novo synthesis of pantothenic acid, persisted in SCID mice, without managing to cause the disease. Sambandamurthy, V. K., Wang, X., Chen, B. et al. A pantothenate auxotroph of M. tuberculosis is highly attenuated and protects mice against tuberculosis. Nat Med 2002, 8(10), 1171-1174. Individual leucine auxotrophs are also strongly attenuated and incapable of replication in vivo in SCID mice. Hondalus, M. K., Bardarov, S., Russell, R., Chan, J., Jacobs, W. R., Jr. & Bloom, B. R. Attenuation of and protection induced by a leucine auxotroph of M. tuberculosis. Infect Immun 2000, 68(5), 2888-2898. Therefore, the principle that vaccine strains based on M. tuberculosis can be successfully attenuated whilst retaining genes that are suppressed in M. bovis BCG is now generally accepted.


Prior to U.S. Pat. No. 8,287,886B2, research into more effective vaccines than BCG was based on the notion that loss of virulence with BCG was in itself a factor that contributed to its lack of complete protective efficacy. Behr, M. A., Wilson, M. A., Gill, W. P. et al. Comparative genomics of BCG vaccines by whole-genome DNA microarray. Science 1999, 284(5419), 1520-1523. It was therefore reasoned that new attenuated mutants of M. tuberculosis, with less virulence, could be more effective as vaccines. In this regard, and although it has been indicated that natural infection with M. tuberculosis and vaccination with BCG do not differ in their capacity to bring about protective immunity against tuberculosis. Sampson, S. L., Dascher, C. C., Sambandamurthy, V. K. et al. Protection elicited by a double leucine and pantothenate auxotroph of M. tuberculosis in guinea pigs. Infect Immun 2004, 72(5), 3031-3037, M. tuberculosis infected individuals with latent tuberculosis have a 79% lower risk of progressive tuberculosis after re-infection as compared to uninfected individuals (Andrews 2012. CID 54:784-790). In addition, and taking into account the fact, that most of these individuals might have been vaccinated with BCG, this is indicative that, in practice, there might be a difference in the protective immunity provided by BCG and by M. tuberculosis. This raised questions as to whether or not it was possible to improve BCG by rational attenuation of M. tuberculosis. Within this context, the observation that the mutant M. tuberculosis strain described in U.S. Pat. No. 8,287,886 B2 with the combination of 2 independent mutations, in synthesis of the PhoP protein and in PDIM synthesis, is more attenuated than BCG in the SCID mouse model, even when applied at a dose 10 times higher than that of BCG, and the greater degree of protection than BCG in the guinea pig model, was deemed of particular relevance.


The mutant M. tuberculosis strain described in U.S. Pat. No. 8,287,886 B2 was characterized by being an isolated microorganism belonging to the Mycobacterium genus, comprising the inactivation of the Rv 0757 (phoP) gene and the inactivation of a second gene that prevented PDIM (phthiocerol dimycocerosates) production. In particular, such mutant M. tuberculosis strain described in U.S. Pat. No. 8,287,886B2 (the SO2 strain) was characterized in that it comprised the inactivation of the Rv 0757 (phoP) gene and a second independent mutation of phoP that prevented PDIM production.


It is interesting to note that, as described in U.S. Pat. No. 8,287,886B2, the SO2 strain was not deemed toxic in six guinea pigs that were inoculated with 50 times the vaccine dose in this species. In addition, their survival rate and weight curve was studied. The survival rate was 100% after the 6-month duration of the experiment. FIG. 12 of U.S. Pat. No. 8,287,886B2 shows the observed weight gain in all the animals over the 6 months, showing the non-toxicity of the SO2 strain (Y=weight in grams and X=time in weeks of infection.). In addition, survival rate of vaccinated guinea pigs after infection with M. tuberculosis was also studied in U.S. Pat. No. 8,287,886B2 (FIG. 13). The protection study in guinea pigs tracked the survival rate of guinea pigs after 300 days. The survival rate curve was measured for unvaccinated guinea pigs (saline) and those vaccinated with the current BCG vaccine, with a M. tuberculosis phoP− strain or with the SO2 strain (phoP− and PDIM− mutant). After subcutaneous vaccination, the animals were infected with a virulent strain of M. tuberculosis (H37Rv) at a high dose to study the survival rate. After 60 days, the 6 guinea pigs that had not been vaccinated (saline) had died, whilst the groups vaccinated with the SO2 strain, phoP− and BCG had survived. After 300 days of infection 3 guinea pigs vaccinated with BCG and phoP− had died, compared to only one of the groups vaccinated with the SO2 strain, which indicates that the protection of the phoP mutant is similar to that of the current vaccine BCG, whereas vaccination with the SO2 strain, the phoP− and PDIM− double mutant, protected better in the guinea pig model. Furthermore, FIG. 14 of U.S. Pat. No. 8,287,886B2 shows the survival after 400 days of the guinea pigs tracked in FIG. 13. The 6 unvaccinated guinea pigs had died after 60 days. After 400 days of infection 3 guinea pigs from the group vaccinated with the SO2 strain (FIG. 14a) survived, whereas just 1 guinea pig vaccinated with BCG (FIG. 14a and FIG. 14b) and phoP− (FIG. 14b) had survived, indicating again that the protection of the phoP mutant is similar to that of BCG, whilst vaccination with the SO2 strain, the phoP− and PDIM− double mutant, protects better after the 400 days of the experiment.


In conclusion, the results described in U.S. Pat. No. 8,287,886B2 show that the SO2 strain and therefore a microorganism belonging to the Mycobacterium genus (particularly from the M. tuberculosis complex) with PhoP− PDIM− phenotype is a more effective vaccine than BCG in accordance with a number of criteria. It is more attenuated than BCG in SCID mice, it provides mice with a protective immunity that is at least as good as BCG and it generates stronger cellular immune responses. Additionally, in protection experiments conducted in guinea pigs against infection with high doses of H37Rv, the strain with phenotype PDIM− PhoP− results in a 100% survival rate of guinea pigs in circumstances in which BCG only achieved a 33% survival rate. This protection is linked to a reduction in the severity of the disease and the bacterial load.


In light of these results, the authors of the present invention proceeded to develop a live-attenuated M. tuberculosis vaccine comprising the MTBVAC strain presented as a lyophilised pellet in amber-glass vials of 3 mL. As already indicated, the MTBVAC strain was constructed to contain two independent non-reverting deletion mutations, without antibiotic markers, fulfilling the first Geneva consensus safety requirements. In this sense, the MTBVAC strain was genetically engineered to phenotypically and functionally resemble its prototype SO2. In the MTBVAC strain, the introduction of an unmarked deletion in fadD26 ensures a genetically stable abolishment of PDIM biosynthesis. It is noted that SO2 has a thorough and complete preclinical history demonstrating robust safety and attenuation profile and promising efficacy compared to BCG in relevant animal models. As already indicated, most of these preclinical studies have been reproduced with MTBVAC to confirm functional profile and biological activity of the double attenuating PhoP−/PDIM−deficient phenotype.


On the basis of the above, the authors of the present invention prepared a vaccine comprising the MTBVAC strain. One dose of 0.05 mL of said vaccine was to be given by using the intradermal route to newborns similarly to BCG. A first objective of the authors of the present invention was thus to obtain a, preferably lyophilized, vaccine useful in neonates for the treatment or prevention of TB in this specific age group population. With that in mind, they conducted, in neonates, the experiments described in examples 2 and 3 of the present application, wherein as a result of these experiments, it was concluded that vaccination with MTBVAC at the estimated dosages of 2.5×104 or 2.5×105 or more CFUs, was immunogenic in neonates from a TB endemic setting.


It is noted that in the present application, the term “neonates” is understood as a newborn child (or other mammal) or as an infant less than four weeks old.


In virtue of the above results, we are currently undertaking a Phase 2a Randomised Controlled Dose-defining Trial of the Safety and Immunogenicity of MTBVAC in healthy, BCG naïve, HIV unexposed, South African newborns. This study will be performed in a population of ninety-nine HIV unexposed, BCG naïve newborns without known household exposure to M. tuberculosis. The estimated study duration (first participant vaccinated to completion of data collection) will be approximately 36 months. In this study, MTBVAC will be administered to the neonates at three dose levels: 1.5-8.5×104 CFU/0.05 ml, 1.5-8.5×105 CFU/0.05 ml and 1.5-8.5×106 CFU/0.05 ml. The active control is the BCG vaccine. Participants will receive a single dose of MTBVAC or BCG administered intradermally on Study Day 0. The objectives of this study are as follows:


Primary:





    • To evaluate safety and reactogenicity of MTBVAC at escalating dose levels compared to BCG vaccine in healthy, BCG naïve, HIV unexposed, South African newborns.

    • To evaluate the immunogenicity of MTBVAC at escalating dose levels in healthy, BCG naïve, HIV unexposed, South African newborns.





Secondary:





    • To evaluate QuantiFERON-TB Gold Plus (QFT) conversion rate in neonates receiving escalating dose levels of MTBVAC.





Exploratory:





    • To evaluate differences in major histocompatibility (MHC)-restricted T-cell responses induced by MTBVAC and BCG vaccination.

    • To evaluate differences in donor-unrestricted T-cell responses induced by MTBVAC and BCG vaccination.





Taking into account the fact that examples 2 and 3 already indicate that vaccination with MTBVAC at the estimated dosages of 2.5×104 or 2.5×105 or more CFUs were immunogenic in neonates from a TB endemic setting, and that the reactogenicity of the MTBVAC vaccine was clearly lower than the reactogenicity produced with the BCG vaccine, it appears plausible that administration of MTBVAC to neonates at doses of 1.5-8.5×104 CFU/0.05 ml, 1.5-8.5×105 CFU/0.05 ml or 1.5-8.5×106 CFU/0.05 ml, would be useful as a prophylactic agent to neonates at risk of infection with M. tuberculosis or those at risk of developing tuberculosis disease.


Therefore, in a first aspect, the invention refers to a composition comprising an isolated microorganism belonging to the M. tuberculosis complex, preferably a M. tuberculosis clinical isolate, more preferably a M. tuberculosis clinical isolate, characterized in that it comprises a PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype), more preferably said microorganism is the MTBVAC strain, wherein the composition comprises at least 1.5×104 cfu/0.05 ml or more of the isolated microorganisms. Preferably, the composition comprises between 1.5×104 cfu/0.05 ml and 8.5×106 cfu/0.05 ml isolated microorganisms. More preferably, the composition comprises between 1.5-8.5×104 cfu/0.05 ml, or between 1.5-8.5×105 cfu/0.05 ml or between 1.5-8.5×106 cfu/0.05 ml of the isolated microorganisms.


In a second aspect of the invention, the composition of the first aspect is administered for prophylaxis in neonates at risk of infection with M. tuberculosis or those at risk of developing tuberculosis disease, against infections caused by M. tuberculosis complex, preferably M. tuberculosis; or for use in the prophylaxis or prevention in neonate humans at risk of developing tuberculosis disease and suffering from latent tuberculosis infection, against the development of the clinical symptomatology associated with the active form of the disease caused by M. tuberculosis complex, preferably M. tuberculosis; or for use as a secondary agent for treating patients infected with latent and/or active TB tuberculosis in neonates; or for use in revaccination, booster vaccination or booster dose in a prophylactic or preventive treatment in neonate humans at risk of infection with M. tuberculosis, against infections caused by M. tuberculosis complex, preferably M. tuberculosis; or for use as a secondary agent for prevention of any unrelated infections other than tuberculosis disease caused by M. tuberculosis, including infection by non-tuberculous mycobacteria in neonates. More preferably, said composition is administered via the intradermal route to the neonates.


In addition to the above, it is further noted that we are currently conducting a double-blind, randomized, BCG-controlled, dose-escalation safety and immunogenicity study in adults with and without latent tuberculosis infection (LTBI), as measured by QuantiFERON-TB Gold Plus (QFT) assay. This is a Phase 1b/2a, double-blind, randomized, BCG-controlled, dose-escalation safety and immunogenicity study in healthy adults with and without LTBI. All participants will have received previous BCG vaccination in infancy. The investigational product is MTBVAC at four dose levels: 5×103 CFU, 5×104 CFU, 5×105 CFU, and 5×106 CFU. The active control is BCG (5×105 CFU).


Participants meeting the inclusion/exclusion criteria will be randomized within a study cohort to receive a single dose of MTBVAC or BCG revaccination administered intradermally on Study Day 0. The study will be conducted at one site in South Africa. Participants will be enrolled into one of eight cohorts and followed for safety and immunogenicity endpoints through Study Day 182. The estimated time to complete enrolment is approximately 9 months.


Cohorts 1-8 will include QFT-negative (Cohorts 1-4) and QFT-positive (Cohorts 5-8) participants. Participants will be randomized within each cohort, to receive either MTBVAC or BCG.


On these bases, in a third aspect, the invention refers to a composition comprising an isolated microorganism belonging to the M. tuberculosis complex, preferably a M. tuberculosis clinical isolate, more preferably M. tuberculosis clinical isolate MT103, characterized in that it comprises a PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype), more preferably said microorganism is the MTBVAC strain, wherein the composition comprises at least 3×103 cfu/0.1 ml or more of the isolated microorganisms. Preferably, the composition comprises between 3×103 CFUs/0.1 ml and 17×106 cfu/0.1 ml of isolated microorganisms. More preferably, the composition comprises between 3-17×103 cfu/0.1 ml, or between 3-17×104 cfu/0.1 ml, or between 3-17×105 cfu/0.1 ml or between 3-17×106 cfu/0.1 ml of the isolated microorganisms.


In a fourth aspect of the invention, the composition of the third aspect is administered for prophylaxis or prevention (including booster vaccination) in non-neonate humans, such as children, adolescents and adults at risk of infection with M. tuberculosis, against infections caused by M. tuberculosis complex, preferably M. tuberculosis. More preferably, said composition is administered via the intradermal route.


In a fifth aspect of the invention, the composition of the third aspect is administered for prophylaxis or prevention in non-neonate humans, such as children, adolescents and adults at risk of developing tuberculosis disease and suffering from latent tuberculosis infection, against the development of the clinical symptomatology associated with the active form of the disease caused by M. tuberculosis complex, preferably M. tuberculosis. More preferably, said composition is administered via the intradermal route.


In a sixth aspect of the invention, the composition of the third aspect is administered for use as a secondary agent for treating patients infected with latent and/or active TB in neonates and non-neonate humans, such as children, adolescents and adults. More preferably, said composition is administered via the intradermal route.


In a seventh aspect of the invention, the composition of the third aspect is administered for booster vaccination or booster dose in a prophylactic or preventive treatment in non-neonate humans, such as children, adolescents and adults at risk of infection with M. tuberculosis, against infections caused by M. tuberculosis complex, preferably M. tuberculosis. In this sense, it is noted that after initial immunization, a booster injection or booster dose is a re-exposure to the immunizing antigen. It is intended to increase immunity against that antigen back to protective levels, after memory against that antigen has declined through time.


On the other hand, the authors of the present invention, in order to achieve a preferred manner of practicing any of the above mentioned aspects of the invention with the MTBVAC strain and of minimizing the loss of viability after lyophilization in a development process that offers consistent results and a product with a shelf life of at least 2 years stored between +2-8° C., carried out numerous studies to establish the most appropriate production process for the MTBVAC vaccine. As a first approximation, different culture media as well as different stabilizer compositions were tested.


The first challenge in the production of the MTBVAC vaccine was to cultivate it in a medium with a defined composition and in which there were no components of animal origin. For this reason, experiments were performed by using the SO2 strain. It is noted, as already mentioned, that the MTBVAC strain was genetically engineered to phenotypically and functionally resemble its prototype SO2, and therefore, the SO2 strain was considered an appropriate starting point to establish the most appropriate production process for the MTBVAC vaccine.


By using the SO2 strain, different media were developed and tested that did not contain any component of animal origin in its composition. Some of the proven culture media were as follows:

    • Middlebrook 7H9 and variations (Media for Tubercle Bacilli, Dubos, R.J. and Middlebrook, G. American Review of Tuberculosis and Pulmonary Diseases, 1947 Vol. 56 No.4 pp. 334-45 ref.15).
    • Sauton synthetic medium (Handbook of Microbiological Media, Fourth Edition, Ronald M. Atlas, CRC Press, 2010. Page 1540) and variations.


The composition of the Sauton and Middlebrook media are detailed in the following tables:









TABLE 1





Sauton


















Glycerol

2%




L-Asparagine
0.4%



Glucose
0.2%



Citric acid
0.2%



Monopotassium phosphate
0.05% 



Magnesium sulphate
0.055% 



Polysorbate 80
0.0155%  



Ammonium ferric citrate
0.005% 



Zinc sulfate
0.00001%  
















TABLE 2





Middlebrook 7H9 + ADC + Polysorbate



















Disodium phosphate
2.5
g/L



Monopotassium phosphate
1.0
g/L



Glutamic acid
0.5
g/L



Ammonium sulfate
0.5
g/L



Sodium citrate
0.1
g/L



Magnesium sulphate
50.0
mg/L



Ammonium ferric citrate
40.0
mg/L



Zinc sulfate
1.0
mg/L



Copper sulphate
1.0
mg/L



Pyridoxine
1.0
mg/L



Calcium chloride
0.5
mg/L



Biotin
0.5
mg/L



Glycerol
2.0
mL/L



Bovine albumin
5.0
g/L



Dextrose
2.0
g/L



Catalase
3.0
mg/L



Polysorbate 80
0.5
g/L









In the Sauton media the growth was similar to the reference medium (Middlebrook medium without modifications, Table 2). FIG. 1 compares the growth curve in Middlebrook with that of the Sauton culture medium. In parallel to the composition of the culture medium, in these tests it began to profile at laboratory scale other variables such as the time of culture, the number of passages of culture and the type of growth, static or in agitation (see Table 3)









TABLE 3







Growth of M. tuberculosis SO2 in Sauton Medium









Culture




conditions
Static
Agitation















Lot
006
008
005
009
011
007
010
012


















Days of
7
10
15
23
24
28
24
31


culture










Viable
9.70 × 107
3.00 × 108
1.91 × 108
1.25 × 108
1.69 × 108
4.70 × 108
3.30 × 106
5.10 × 106


count










(cfu/mL)










Optic
0.475
0.666
1.86
2.56
2.17
2.92
0.408
0.198


density










(600 nm)









Finally, the Sauton Synthetic medium was selected under static growth conditions, as it is valid for growing the SO2 strain. Non-static growth conditions could have also been selected, however, the culture needs to be under aerobic conditions.


The next step of the development was to study the lyophilization process. Lyophilization is a critical step in the production of a live vaccine. Achieving the stability of lyophilized vaccines is a complex process, since microorganisms are not only susceptible to environmental factors after lyophilization, such as temperature, but growth and formulation conditions can also affect the success of the process. The yield of viable bacteria after lyophilization and subsequent storage stability may be affected by factors such as lyophilization cycle, stabilizer composition, residual moisture and the presence of air.


In the development phase with SO2, up to 11 different stabilizer compositions were tested. The following table illustrates the stabilizer compositions tested:












TABLE 4






Stabilizer
Components
Concentration








S
Medium (no stabilizer)
NA












G
Sodium glutamate
10-40
g/L



GSA
Sodium glutamate
10-40
g/L




Sucrose
100-400
g/L



M
Mannitol
20-50
g/L



MS
Mannitol
20-50
g/L




Sucrose
100-400
g/L



GSM
Sodium glutamate
10-40
g/L




Sucrose
100-400
g/L




Mannitol
20-50
g/L



GC
Glycocola
30-200
g/L




Trisodium citrate
30-40
g/L



GSb
Glycocola
30-200
g/L




Sucrose
100-400
g/L



GT
Glycocola
30-200
g/L




Trehalose
18-60
g/L



CGS
Trisodium citrate
30-40
g/L




Glycocola
30-200
g/L




Sucrose
100-400
g/L



CFT
Sodium chloride
2-5
g/L




Monopotassium phosphate
2-5
g/L




Trehalose
60
g/L









In the stabilizer studies different formulations were also tested, varying in addition to the compositions the proportions of the stabilizer and culture medium, as well as the volume of lyophilization. In all the tests, the viability loss in the lyophilized product and the stability after 30 days at 37° was determined. As a criterion for selecting the stabilizers for future tests, a limit of viability loss of 90% and/or a maximum of 80% loss after the accelerated stability test at 37° C. was established (see results in table 5).









TABLE 5







Lyophilization of SO2 with different stabilizers.









Stabilizer




















Batch
Specification
GSA
G
GSM
M
MS
GSB
GC
GS
CGS
CFT
GT
S























005
% loss
29%
53%









 84%



lyophilization















% loss at
90%
>99% 









>99%



37° C.














006
% loss
7.40%
10%
 8%
66%
5.00%






>99%



lyophilization















% loss at
87%
61%
66%
99%
97.7%






Nd



37° C.














007
% loss
65%

53%
99%











lyophilization















% loss at
98.5%

92.3%
>99% 











37° C.














008
% loss
24%

12%
67%











lyophilization















% loss at
88%

88%
>99% 











37° C.














009
% loss
31%

20%
77%











lyophilization















% loss at
85%

>99% 
>99% 











37° C.














010
% loss
70%


91%

 54%
 79%








lyophilization















% loss at
88.5%


>99% 

>99%
>99%








37° C.














011
% loss
9.40%






 61%







lyophilization















% loss at
57%






>99%







37° C.














012
% loss
84%




 97%


 95%
 98%
>99%




lyophilization















% loss at
>99% 




>99%


>99%
>99%
>99%




37° C.









After the above mentioned preliminary trials, it was concluded that it was necessary to add a stabilizer to the culture medium to lyophilize, since the losses in lyophilization without stabilizer were greater than 99%, and the best stabilizer to meet the specification for lyophilization loss and the specification for accelerated stability at 37° C., was GSA (Sodium glutamate and Sucrose).


After reaching the above conclusions, the MTBVAC strain was received in the form of a freeze-dried Pre-master seed lot, and shortly after, we began the cell cultures of this particular strain. For the growth of the MTBVAC strain, first Sauton media with the same composition as that used in the growth studies of the parental strain SO2 (see table 1) was used. However, unexpectedly, in the case of MTBVAC, a lower growth was observed in Sauton synthetic medium than that observed for the SO2 strain. In addition, problems in the amplification phase of the MTBVAC strain were also detected. In order to solve these problems, tests were performed adding and eliminating components from the Sauton media composition. Such modifications consisted on the addition or elimination of supplements such as glucose, zinc sulphate, biotin, glycerol and polysorbate.


The enrichment of the Sauton synthetic medium with zinc sulfate and biotin did not offer good results and no growth of MTBVAC was observed. In the case of enrichment with glucose, polysorbate and glycerin, the results were favorable and an adequate growth of MTBVAC was obtained.


As a result of these growth studies SD and SDG media were developed and the MTBVAC cultures were grown in these media. The growth of MTBVAC was good both in SD medium and in SDG medium, but some cultures were stopped after successive passages in SDG medium, so the SD medium was the one selected for the amplification passages. FIG. 2 shows the OD results of the MTBVAC cultures in Sauton, SD and SDG media.


However, when cultures of the MTBVAC strain were initiated from vials of the lyophilized or freezed-dried Master seed lot, it was observed that the growth could not be initiated in the SD medium, so modifications were made in the composition thereof and a seed medium was developed. As a conclusion of these studies and for future pilot and industrial tests as a means to start the cultures, the seed medium was selected, as a means for the amplification passages the SD medium was selected, and as a means for the mass culture before lyophilization, the SDG medium was selected. In addition, it is important to note that the composition of the SD medium in combination with the stabilizer affected the lyophilization process and the appearance of the tablet, therefore the lyophilization process will only be performed in the SDG medium.


We herein provide the composition of the Seed, SD and SDG media.












TABLE 6






Seed
SD
SDG


Components
medium
medium
medium





















L-Asparagine
2.00-4.00
g
2.00-4.00
g
2.00-4.00
g


Monopotassium
0.30-0.60
g
0.30-0.60
g
0.30-0.60
g


phosphate








Magnesium
0.5-0.70
g
0.50-0.70
g
0.50-0.70
g


sulfate H2O








Ammonium
0.02-0.05
g
0.02-0.05
g
0.02-0.05
g


ferric citrate








Dextrose
7.00-8.00
g
3.00-4.00
g
3.00-4.00
g


monohydrate








Glycerol
10.0-20.0
mL
30-40
mL
3.0-10.0
mL


Citric acid
1.5-2.0
g
1.5-2
g
1.5-2
g


Polysorbate 80


0.15-0.5
mL
0.15-0.5
mL


Purified water QS
1.00
L
1.00
L
1.00
L









In this sense, the following three tables show the results of the industrial scale production of five batches of MTBVAC 2.5×105 that demonstrate the consistency of the results obtained with the means developed in the study.









TABLE 7







Culture of MTBVAC from the lyophilized working seed-bank in seed medium












Control
Lot 170928
Lot 170580
Lot 171811
Lot171911
Lot 172547





Culture appearance
conformable
conformable
conformable
conformable
conformable


Purity
Absence of
Absence of
Absence of
Absence of
Absence of


(EP 2.6.1)
contamination
contamination
contamination
contamination
contamination


Purity (Ziehl-
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol


Neelsen)
resistant
resistant
resistant
resistant
resistant



bacilli
bacilli
bacilli
bacilli
bacilli


Viable bacteria
1.37 × 106
5.3 × 106
5.4 × 106
7.5 × 106
1 × 106


count
cfu/mL
cfu/mL
cfu/mL
cfu/mL
cfu/mL
















TABLE 8







Culture of MTBVAC in SD medium from the previous passage (Table 7)












Control
Lot 170928
Lot 170580
Lot 171811
Lot 171911
Lot 172547





Culture Appearance
conformable
conformable
conformable
conformable
conformable


Purity
Absence of
Absence of
Absence of
Absence of
Absence of


(EP 2.6.1)
contamination
contamination
contamination
contamination
contamination


Purity (Ziehl-
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol


Neelsen)
resistant
resistant
resistant
resistant
resistant



bacilli
bacilli
bacilli
bacilli
bacilli


Viable bacteria count
6.04 × 108
4.33 × 108
1.16 × 108
3.16 × 108
3.26 × 108



cfu/mL
cfu/mL
cfu/mL
cfu/mL
cfu/mL
















TABLE 9







Culture of MTBVAC in SD medium from the previous passage (Table 8)












Control
Lot 170928
Lot 170580
Lot 171811
Lot 171911
Lot 172547





Culture Appearance
conformable
conformable
conformable
conformable
conformable


Purity
Absence of
Absence of
Absence of
Absence of
Absence of


(EP 2.6.1)
contamination
contamination
contamination
contamination
contamination


Purity (Ziehl-
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol


Neelsen)
resistant
resistant
resistant
resistant
resistant



bacilli
bacilli
bacilli
bacilli
bacilli


Viable bacteria count
1.73 × 108
3.03 × 108
3.02 × 108
1.27 × 108
3.7 × 108



cfu/mL
cfu/mL
cfu/mL
cfu/mL
cfu/mL
















TABLE 10







Culture of MTBVAC in SDG medium from the previous passage (Table 9)












Control
Lot 170928
Lot 170580
Lot 171811
Lot171911
Lot 172547





Culture Appearance
conformable
conformable
conformable
conformable
conformable


Purity
Absence of
Absence of
Absence of
Absence of
Absence of


(EP 2.6.1)
contamination
contamination
contamination
contamination
contamination


Purity
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol
Acid-alcohol


(Ziehl-
resistant
resistant
resistant
resistant
resistant


Neelsen)
bacilli
bacilli
bacilli
bacilli
bacilli


Viable bacteria
7.1 × 108
4.33 × 108
4.51 × 108
2.77 × 108
3.26 × 108


count
cfu/mL
cfu/mL
cfu/mL
cfu/mL
cfu/mL









In the previous indicated studies of development with the SO2 strain, we concluded that in the lyophilization process it was necessary to use a stabilizer to reduce the losses of viable bacteria count and to improve the stability of the lyophilized product. For the development of MTBVAC, the same stabilizers selected in the study with SO2 were used. The objective was to obtain a lyophilized vaccine with a concentration ranging from 3×103 cfu/0.1 ml and 17×106 cfu/0.1 ml, preferably ranging from 3-17×103 cfu/0.1 ml, or between 3-17×104 cfu/0.1 ml, or between 3-17×105 cfu/0.1 ml or between 3-17×106 cfu/0.1 ml of the MTBVAC strain, minimizing the loss of viability after lyophilization in a development process that offered consistent results and a product with a shelf life of at least 2 years stored between 2-8° C.


In the development phase with MTBVAC, up to 7 different stabilizer compositions were tested. The following table 11 illustrates the stabilizer compositions tested:












TABLE 11






Stabilizer
Components
Concentration








S
Medium (no stabilizer)
NA












GSA
Sodium glutamate
10-40
g/L




Sucrose
100-400
g/L



GSM
Sodium glutamate
10-40
g/L




Sucrose
100-400
g/L




Mannitol
20-50
g/L



GSb
Glycocola
30-200
g/L




Sucrose
100-400
g/L



GT
Glycocola
30-200
g/L




Trehalose
18-60
g/L



GTS
Trehalose
30-60
g/L




Glycocola
40-100
g/L




Sucrose
75-200
g/L



GSTG
Sodium glutamate
10-40
g/L




Glycocola
75-150
g/L




Sucrose
75-200
g/L




Trehalose
15-60
g/L









The following tables below 12 to 13 show the results in terms of percentage of viability loss in an accelerated stability study of laboratory-scale lyophilization tests of MTBVAC. The tables show the effect of the composition of the lyophilization medium in combination with the stabilizer in the lyophilization process. From these studies it was concluded that it is necessary to add stabilizer for the lyophilization of MTBVAC and that the GSA stabilizer is the one that offers the best results for the parameters tested.









TABLE 12







Lyophilization of MTBVAC grown in SD medium with


different stabilizers. Percentage of viability


loss in an accelerated stability study.














Batch
GSA
GSB
GSM
GT
S






001
 73%
97%

>99%




005
>99%







009
>99%



>99%



011
>99%







012
>99%







013
>99%


>99%
>99%



014
>99%

>99%
















TABLE 13







Lyophilization of MTBVAC grown in SDG medium


with different stabilizers. Percentage of viability


loss in an accelerated stability study.














Batch
GSA
GSB
GSM
GTS
GT
GSTG
S





002
61%
>99%

60%
 98%
98%



003
62%

77%






004
89%



>99%

>99%


005
73%








006
59%

>99% 






007
49%

32%
86%









Lastly, the following table shows the lyophilization results of 4 batches of MTBVAC:














TABLE 14





Control
Specification
Lot 102897
Lot 110142
Lot 110238
Lot 110380







Appearance
Lyophilized pill
conform
conform
conform
conform


Vacuum
Complies
conformable
conformable
conformable
conformable


Purity
Absence of
conformable
conformable
conformable
conformable


(EP 2.6.1)
contamination






Residual moisture
<3% w/w
1.44%
1.26%
1.68%
1.84%


Identification
Molecular
conform
conform
conform
conform


(PCR)
characterization






Viable count
3-17 × 106
1.63 × 107
8.54 × 106
1.58 × 107
8.54 × 106


(cfu/vial)
cfu/vial






Lyophilization loss
<90%
  64%
  67%
  63%
  67%









FIG. 3 shows the stability results between 2-8° C. and −30° C. of the lots or batches identified in table 14 above. Moreover, the following table 15 provides further results of parallel lyophilization of the culture of table 11 (SDG medium) in a pilot and industrial plant.










TABLE 15








Lyophilization lot














Control
Specification
171437P
171611In
171889P
171976In
172952P
172871IN

















Culture lot

170928
170928
170580
170580
172547
172547


MTBVAC









Appearance
Lyophilized pill
conformable
conformable
conformable
conformable
conformable
conformable


Vacuum
Complies
conformable
conformable
conformable
conformable
conformable
conformable


Purity
Absence of
conformable
conformable
conformable
conformable
conformable
conformable


(EP 2.6.1)
contamination








Residual
<3% w/w
1.72
1.89
2.02
2.13
1.89
1.37


moisture









Identification
Molecular
conformable
conformable
conformable
conformable
conformable
conformable


(PCR)
characterization








Viable count
3-17 × 106 cfu/vial
1.5 × 107
1.6 × 107
6.03 × 107
1.17 × 107
1.03 × 107
1.37 × 107


(cfu/vial)









Lyophilization
<90%
64%
67%
63%
67%
81.03%
74.76%


loss









All of the above results were obtained by the lyophilisation of the SDG medium in which the MTBVAC strains were grown, preferably grown in the range between 1×108 to 5×108 cfu/mL. It is noted that to carry out said lyophilisation, sodium glutamate and sucrose (GSA) was added, preferably at a concentration between 10-40 g/L of sodium glutamate and between 100-400 g/L of sucrose.


Therefore, described herein are specific formulations and methods that can be used for the preparation of live MTBVAC strain-based pharmaceutical products, as described further below. The formulations of the invention comprise or consist of any of the compositions detailed below per se and these may be use for culturing MTBVAC strains. The compositions are detailed below:















Components
Seed medium
Medium SD
Medium SDG





















L-Asparagine
2.00-4.00
g
2.00-4.00
g
2.00-4.00
g


Monopotassium
0.30-0.60
g
0.30-0.60
g
0.30-0.60
g


phosphate








Magnesium
 0.5-0.70
g
0.50-0.70
g
0.50-0.70
g


sulfate H2O








Ammonium
0.02-0.05
g
0.02-0.05
g
0.02-0.05
g


ferric citrate








Dextrose monohydrate
7.00-8.00
g
3.00-4.00
g
3.00-4.00
g


Glycerol
10.0-20.0
mL
30-40
mL
 3.0-10.0
mL


Citric acid
1.5-2.0
g
1.5-2
g
1.5-2
g


Polysorbate 80


0.15-0.5 
mL
0.15-0.5 
mL


Purified water QS
1.00
L
1.00
L
1.00
L









Thus, an eighth aspect of the invention refers to a composition comprising or consisting of the seed medium as characterized above.


A ninth aspect of the invention refers to a composition comprising or consisting of the SD medium as characterized above.


A tenth aspect of the invention refers to a composition comprising or consisting of the SDG medium as characterized above.


An eleventh aspect of the invention refers to any of the seed medium, the SD medium or the SDG medium, as characterized above, wherein said medium further comprises MTBVAC strains grown therein, preferably in the range between 1×108 to 5×108 cfu/mL.


A twelve aspect of the invention refers to the use of any of the seed medium, the SD medium or the SDG medium, as characterized above, for culturing or expanding MTBVAC strains, under aerobic conditions. In this sense, preferably as a means to start the MTBVAC strain cultures, the seed medium is selected, as a means for the amplification passages the SD medium is selected, and as a means for the mass culture before lyophilization, the SDG medium is selected. In particularly preferred embodiments of the twelve aspect of the invention, the invention refers to a process for the production of a ready to freeze-dried live-attenuated M. tuberculosis vaccine composition comprising an isolated microorganism belonging to a M. tuberculosis strain having a i) PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and ii) the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype), much preferably the MTBVAC strain, wherein the process comprises starting the culture of the M. tuberculosis strain and expanding or amplifying said bacteria by using a suitable cell medium, wherein the process is characterized in that for the mass culture before lyophilization, a SDG medium is used. Preferably, the process comprises starting the culture of the M. tuberculosis strain in the seed medium and expanding or amplifying said bacteria by using the SD medium, and using the SDG medium for the mass culture before lyophilization. More preferably, the process further comprises a freeze-drying step by adding sucrose and sodium glutamate as stabilizers to the SDG medium used for the mass culture prior to the lyophilization step.


In addition, certain components (e.g., particular stabilizers, bulking agents, and buffers) have been found to be advantageous in the preparation of lyophilized MTBVAC strains vaccines. The invention also relates to reconstituted vaccines, and prophylactic and therapeutic methods employing the compositions described herein. The compositions and methods of the invention are described further, as follows.


In particular, a thirteenth aspect of the invention provides a live-attenuated M. tuberculosis vaccine composition comprising an isolated microorganism belonging to a M. tuberculosis strain having a i) PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and ii) the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype), preferably the M. tuberculosis strain is the MTBVAC strain, wherein said composition is a freeze-dried composition, and wherein said composition is obtained by freeze-drying a culture medium comprising the microorganism by adding sucrose and sodium glutamate as stabilizers, and wherein the culture medium is the SDG medium. More preferably, in a thirteenth aspect, the present invention provides a live-attenuated M. tuberculosis vaccine composition comprising an isolated microorganism belonging to a M. tuberculosis strain having a i) PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and ii) the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype), wherein preferably the M. tuberculosis strain is the MTBVAC strain, and wherein said live-attenuated M. tuberculosis vaccine composition is obtained or obtainable according to the process of the twelve aspect of the invention.


Still more preferably, the present invention provides a live-attenuated M. tuberculosis vaccine composition, preferably a reconstituted composition after freeze-drying, comprising an isolated microorganism belonging to a M. tuberculosis strain having a i) PhoP− phenotype by the inactivation by a genetic deletion of the Rv0757 gene and ii) the deletion of a second gene, Rv2930 (fadD26), that prevents PDIM production (PDIM− phenotype), wherein preferably the M. tuberculosis strain is the MTBVAC strain, and wherein said composition is characterized in that it comprises or consists of the following components per mL (in percentual terms):
















MTBVAC



Components
Dose per 1 mL








L-Asparagine
0.034-0.066%



Monopotassium
0.006-0.010%



phosphate




Magnesium
0.008-0.012%



sulfate H2O




Ammonium
0.0004-0.0008%



ferric citrate




Dextrose
 0.05-0.066%



monohydrate




Glycerol
0.00005-0.0001% 



Citric acid
0.026-0.034%



Polysorbate 80
0.000002-0.000008%



Sodium
0.33-1.33%



glutamate




Sucrose
 3.3-13.3%



Purified
1 mL



water QS









More preferably, the live-attenuated M. tuberculosis vaccine composition mentioned in the paragraph above is freeze-dried, or a reconstituted composition obtained by adding water, preferably sterilized water for injection, to a freeze-dried composition.


In a preferred embodiment of the thirteenth aspect of the invention or of any of its preferred embodiments, said composition is characterized in that it comprises at least 3×103 cfu per 0.1 ml, preferably per 0.1 ml of water, or more strains of the microorganism. Preferably, the composition comprises between 3×104 cfu per 0.1 ml and 17×106 cfu per 0.1 ml strains of the isolated microorganism. More preferably, the composition comprises between 3 and 17×104 cfu per 0.1 ml, or between 3 and 17×105 cfu per 0.1 ml or between 3 and 17×106 cfu per 0.1 ml strains of the isolated microorganism. Still more preferably, release specification for the freeze-dried MTBVAC vaccine comprising between 1.5 and 8.5×105 cfu/0.05 ml MTBVAC strains, is detailed in the table below














Test
Acceptance Criteria
Methodology







Appearance
White freeze dried pellet
Observation


Vacuum
Any vial without vacuum is
Fluorescence is



discarded.
observed


Purity
Absence of bacterial and fungal
Eur. Ph. Sterility



contamination except for the
test (2.6.1)



presence of mycobacteria.



Water
≤3% w/w
Karl-Fischer




method


Identification-PCR
Confirmation of fadD26
Real-time PCR



and phoP deletions
assay


Viable bacterial
1.5-8.5 × 105
Counting in


count
cfu/dose (0.05 ml)
Specific




medium


Loss on drying
≤90%
Loss of viability


Excessive dermal
Reaction is lower than from that
Eur. Ph. BCG


reactivity
produced by the
(0163) test



comparison vaccine



Virulent
Not more than 1
Eur. Ph. BCG


mycobacteria
from 10 animals
(0163) test



dies during the 42 days




following the injection,




and autopsy does not reveal




any sign of tuberculosis.



Presentation
Complies
Check of the




packaging









In addition, as shown in this specification, stability data demonstrates that both master and working cell banks, prepared from the Pre-master seed, are stable (see FIG. 9) and that the vaccine MTBVAC stored between −15° C.-30° C. and between +2-+8° C. is stable for more than 24 months (see FIGS. 3 and 10A-10B).


In addition, in use stability study shows that MTBVAC vaccine is stable for at least 8 hours at room temperature once it has been reconstituted.


As is discussed in further detail elsewhere herein, the compositions of the invention are particularly advantageous because of the stability and viability of the active components, which is due in large part to the formulation and the process by which the product is prepared, which involves lyophilization. In general, this process includes the following steps: freezing, primary drying, secondary drying, and stoppering. The process is described in further detail below, in the experimental examples, but an example of the process is as follows. In the freezing step, the lyophilizer shelves are pre-cooled to −50° C. Once all trays are loaded, the shelves are held at −50° C. for 120 minutes. In the primary drying step, the vacuum is set to 25 mT, and the following ramp steps are carried out: ramp at +0.1° C./minute to a shelf temperature of −40° C., hold for 500 minutes; ramp at +0.1° C./minute to a shelf temperature of −35° C., hold for 500 minutes; ramp at +0.1° C./minute to a shelf temperature of −30° C., hold for 500 minutes, and ramp at +0.1° C./minute to a shelf temperature of −25° C., hold for 800 minutes. In the secondary drying step, the vacuum remains at 25 mT, and a ramp step is carried out such that ramping is at +0.1° C./minute to a shelf temperature of +20° C., hold for 800 minutes. If necessary, the product can be held at +20° C., 25 mT up to 24 additional hours before stoppering. In the stoppering step, the chamber is outgassed with 0.22 μm filtered, dry, nitrogen gas, the vacuum is set to 800 mbar (slight vacuum), and stoppers are pushed into vials. Alternative lyophilization cycles that can be used in the invention are well known in the art. Thus, the methods of the invention can involve freezing at or to about, for example, −70° C. to −30° C. (e.g., −60° C. to −40° C., or −50° C.). The freezing can be carried out for about 30 to 240 minutes (e.g., 60 to 120 minutes) or longer. The material can then be subject to one or more drying steps, as described herein. In these steps, a vacuum can be applied (e.g., 25 mT) and the temperature can be changed gradually (e.g., 0.1 to 1.0° C./minute, or 0.5° C./minute), over the course of a period of time (such as, 100-1000 minutes, e.g., 200-600 or 300-500 minutes). In the primary drying, the temperature may be raised to or about, for example, −30° C. to +10° C., e.g., −20° C. to +5° C. or −15° C. to 0° C., while in the secondary drying, the temperature may be changed to, for example, +5° C. to +35° C., e.g., 10° C. to 30° C., or 15° C. to 20° C. As is known to those skilled in this art, these parameters (e.g., temperatures, hold times, ramp rates, and vacuum levels) can be changed based on, for example, results obtained.


The vaccine compositions of the thirteenth aspect of the invention can be administered, according to a fourteenth aspect of the invention, as primary prophylactic agents to those at risk of infection with M. tuberculosis or those at risk of developing tuberculosis disease, or can be used as secondary agents for treating infected patients. Because the strains of these compositions are attenuated, they are particularly well suited for administration to “at risk individuals” such as newborns, children, adolescents, adults, and elderly. Such vaccines can also be used in veterinary contexts.


A preferred embodiment of the fourteenth aspect of the invention relates to the MTBVAC vaccine for immunizing an individual against the symptoms caused by tuberculosis. It is noted that said vaccine may be also suitable for the treatment of bladder cancer as well as for the treatment or prevention of TB, or as a vector or adjuvant. Preferably to immunize an individual against the symptoms caused by TB.


In another preferred embodiment of the fourteenth aspect of the invention, the composition of the thirteenth aspect is administered for prophylaxis in neonates at risk of infection with M. tuberculosis or those at risk of developing TB disease, against infections caused by M. tuberculosis complex, preferably M. tuberculosis. More preferably, said composition is administered via the intradermal route to the neonates.


In another preferred embodiment of the fourteenth aspect of the invention, the composition of the thirteenth aspect is administered for prophylaxis or prevention (including booster vaccination) in non-neonate humans, such as children, adolescents and adults at risk of infection with M. tuberculosis, against infections caused by M. tuberculosis complex, preferably M. tuberculosis. More preferably, said composition is administered via the intradermal route.


In another preferred embodiment of the fourteenth aspect of the invention, the composition of the thirteenth aspect is administered for prophylaxis or prevention in non-neonate humans, such as children, adolescents and adults at risk of developing TB disease and suffering from latent tuberculosis infection, against the development of the clinical symptomatology associated with the active form of the disease caused by M. tuberculosis complex, preferably M. tuberculosis. More preferably, said composition is administered via the intradermal route.


In another preferred embodiment of the fourteenth aspect of the invention, the composition of the thirteenth aspect is administered for use as a secondary agent for treating patients infected with latent and/or active TB in neonates and non-neonate humans, such as children, adolescents and adults. More preferably, said composition is administered via the intradermal route.


In another preferred embodiment of the fourteenth aspect of the invention, the composition of the thirteenth aspect is administered for booster vaccination or booster dose in a prophylactic or preventive treatment in non-neonate humans, such as children, adolescents and adults at risk of infection with M. tuberculosis, against infections caused by M. tuberculosis complex, preferably M. tuberculosis. In this sense, it is noted that after initial immunization, a booster injection or booster dose is a re-exposure to the immunizing antigen. It is intended to increase immunity against that antigen back to protective levels, after memory against that antigen has declined through time.


Throughout the description and claims the word “comprise” and its variants do not imply the exclusion of other technical characteristics, additives, components or steps. For a person skilled in the art, other objects, advantages and characteristics of the invention will arise partly out of the description and partly when the invention is put into practice. The following examples and figures are provided by way of a non-limiting, illustrative example of the present invention.


EXAMPLES
Example 1. Immunogenicity and Protection are Independent of the Dose of MTBVAC in Newborn Mice

Newborn C3H mice (1-to-3 days old) were vaccinated intradermally with 25 μl containing one clinical dose of BCG (2.5×105 aprox), or the indicated CFU dosages of MTBVAC. For BCG groups, commercial vials of BCG Danish were used, corresponding to lots 111053F and 113033C. In the case of MTBVAC, animals were immunized with the MTBVAC vaccine produced by the lyophilisation of the SDG medium in which the MTBVAC strains were grown, to carry out said lyophilisation, sodium glutamate and sucrose (GSA) was added at a concentration between 10-40 g/L of sodium glutamate and between 100-400 g/L of sucrose. Lyophilized formulations were resuspended.


Protective Efficacy Studies

Eight weeks post-vaccination, mice were challenged intranasally with 150 CFU of M. tuberculosis strain H37Rv. Four weeks later, mice were sacrificed and bacterial burden was determined in lungs by tissue homogeneate plating on 7H11S solid medium. The results are shown in FIG. 4.


Immunogenicity Studies

Eight weeks post vaccination, mice were sacrificed and splenocytes isolated for immunogenicity assessment. One million of splenocytes were incubated 24 hours in the presence of 10 μg/ml of Purified Protein Derivative (PPD), 2 μg/ml of overlapping ESAT6 or CFP10 peptides, or non-antigen (negative control). Interferon gamma (IFNγ) producing cells were analyzed by ELISPOT. The results are shown in FIGS. 5A-5C.


Conclusion

Neither protective efficacy nor immunogenicity specific for PPD, ESAT6 or CFP10 induced by MTBVAC was shown to be dose dependent in the newborn mouse model.


Example 2. Phase 1B Immunogenicity Data in Newborns (South Africa)

Objective: We sought to determine immunogenicity and characterize induced immune responses after neonatal vaccination with the MTBVAC vaccine described in the present invention.


Methods: Thirty-six HIV-unexposed, BCG-naïve healthy newborns were randomized 1:3 to receive either BCG (strain SSI) or MTBVAC at 2.5×103, 2.5×104, or 2.5×105 CFU within 96 h of birth. MTBVAC-specific cytokine responses in whole blood were measured on days 7, 28, 70 by whole blood intracellular cytokine staining and flow cytometry on a BD LSRFortessa (18 colour, blue-red-violet-green configuration).


Narrative for Whole Blood ICS Assay:

Fresh whole heparinized bloods were stimulated immediately with BCG, MTBVAC, or phytohemagglutinin (PHA) or were left unstimulated (Nil), for 12 hours at 37° C. Stimulation conditions include half the blood volume [250 μL (0.25 ml)] and only Nil, MTBVAC and BCG. After 7 hours of stimulation, supernatant (for soluble cytokine/chemokine analysis) were collected from all the conditions, frozen at −BOC and stored for shipping to Sponsor for further analysis. Following supernatant removal, brefeldin A was added for the remaining whole blood and tubes incubated for a further 5 hrs in a programmable water bath. The water bath will switch off after a total of 12 hours of stimulation. The next morning, FACS Lysing solution was added to lyse red cells and fix white cells. Fixed, white cells were then frozen for later intracellular cytokine staining and flow cytometry. Flow cytometric staining and acquisition will be run in batches at a later time point. Measurement of frequencies and patterns of specific type-1 cytokines and IL-17 by CD4 T cells were assessed. The timepoints for immunogenicity have been selected on the basis of recent studies conducted by SATVI, which have shown that the peak of the BCG-induced T cell responses in infants is around 6-10 weeks of age.


Results: Vaccination with escalating doses of MTBVAC resulted in predominantly Th1 (IFN-γ, IL-2, or TNF-α) antigen-specific CD4 T-cell responses. The highest MTBVAC dose of 2.5×105 CFU induced the greatest magnitude antigen-specific CD4 T-cells cytokine response at day 70. The lowest MTBVAC dose of 2.5×103 CFU was the least immunogenic. Results are further illustrated in FIG. 6.


Conclusions: These data indicate that vaccination with MTBVAC at 2.5×104 or 2.5×105 or more CFU are immunogenic in neonates from a TB endemic setting.


Example 3

A randomized, double-blind, dose-escalation clinical trial of MTBVAC compared to BCG Vaccine SSI, nd newborns with a safety arm in adults in a living in a TB endemic region


Objectives. Evaluation of safety and immunogenicity of 3 doses of MTBVAC vs BCG in newborns in a TB endemic region.


Methods Eighteen HIV−, QuantiFERON (QFT)−, previously BCG vaccinated healthy adults were randomized 1:1 to receive MTBVAC (5×105 CFU) or BCG SSI. Thereafter, 36 HIV-unexposed, BCG-naïve healthy newborns were randomized 1:3 to receive BCG SSI or MTBVAC at 2.5×103, 2.5×104, or 2.5×105 CFU within 96 h of birth. QFT was performed at D180 and D360 and QFT+ infants (>0.35 IU/mL) were referred for isoniazid preventive therapy.


Results All adults experienced local injection site reactions with swelling in 18 (100%), redness in 16 (88.9%) and ulceration in 10 (55.5%). Nine reactions were reported as moderate and a single swelling event was severe (35 mm). No SAEs were reported at D28.


Unavailability of BCG Vaccine SSI resulted in open-label dosing of 6 infants with MTBVAC at the highest dose. Sixteen (44.4%) infants across all 3 cohorts had local reactions 2 [16.6%], 3 [25%] and 11 [91.6%]), all rated mild with swelling in 14 (38.9%), erythema in 5 (13.9%) and scarring in 9 (25.0%). No ulceration was seen. Systemic AEs were similar across cohorts (n=32/42/40) with 9 graded moderate (n=3/4/2) and 8 severe (n=4/2/2). Six infants experienced 7 unrelated SAEs including an unrelated death due to viral pneumonia, confirmed by autopsy.


Dose-related QFT conversion was noted at D180 in MTBVAC recipients in Cohort 1: (n=3, 37.5%), Cohort 2 (n=6, 75%) and Cohort 3 (n=7, 77.8%), but in zero of 7 BCG recipients. A positive QFT at D360 was seen in 0 Cohort 1 MTBVAC recipients (0.0%), 2 in Cohort 2 (25.0%) and 4 in Cohort 3 (44.4%) as illustrated in FIG. 7.


Conclusion MTBVAC appeared safe at 3 dose levels in South African newborns; and appeared to result in transient dose-dependent QFT conversion, which may be an encouraging indicator of immunogenicity in TB endemic regions. In addition, the reactogenicity of the MTBVAC vaccine was clearly lower than the reactogenicity produced with the BCG vaccine, wherein administration of the BCG vaccine in 5 out of 8 (62%) newly born produces scars, while MTBVAC at its highest dose produced scars in only 2 out of 10 (20%) newly born.

Claims
  • 1.-22. (canceled)
  • 23. A unit dose of an intradermal vaccine composition for intradermal administration to a human neonate, comprising an isolated Mycobacterium tuberculosis bacterium, wherein the M. tuberculosis bacterium comprises a PhoP− phenotype from deletion of the Rv0757 gene and a PDIM− phenotype from deletion of the Rv2930 (fadD26) gene, wherein the isolated M. tuberculosis bacterium is a M. tuberculosis MT103 strain or a M. tuberculosis MTBVAC strain, and wherein the unit dose comprises between 1.5×105 CFU/0.05 ml and 8.5×105 CFU/0.05 ml of the isolated M. tuberculosis bacterium.
  • 24. The unit dose of claim 23, wherein the isolated M. tuberculosis bacterium is the M. tuberculosis MTBVAC strain.
  • 25. The unit dose of claim 23, wherein the isolated M. tuberculosis bacterium is M. tuberculosis MT103.
  • 26. The unit dose of claim 23, wherein the unit dose comprises 2.5×105 CFU/0.05 ml of the isolated M. tuberculosis bacterium.
  • 27. A method of preventing infection with M. tuberculosis complex or tuberculosis disease in a human neonate at risk of infection with M. tuberculosis complex or developing tuberculosis disease, the method comprising intradermal administration of the unit dose of claim 23 to the human neonate.
  • 28. A method of preventing the development of the clinical symptomatology associated with the active form of the tuberculosis disease caused by M. tuberculosis complex in a human neonate at risk of developing tuberculosis disease and suffering from latent tuberculosis infection, the method comprising intradermal administration of the unit dose of claim 23 to the human neonate.
  • 29. A method for treating latent and/or active tuberculosis in a human neonate, the method comprising intradermal administration of the unit dose of claim 23 to the human neonate as a secondary agent.
  • 30. A method of vaccinating a human neonate against infection caused by M. tuberculosis complex, the method comprising intradermal administration of the unit dose of claim 23 to the human neonate as a booster vaccine.
  • 31. A method of preventing an infection other than tuberculosis disease caused by M. tuberculosis, including infection by non-tuberculous mycobacteria, in a human neonate, the method comprising intradermal administration of the unit dose of claim 23 to the human neonate.
  • 32. A unit dose of an intradermal vaccine composition for intradermal administration to a non-neonate human comprising an isolated M. tuberculosis bacterium, wherein the M. tuberculosis bacterium comprises a PhoP− phenotype from deletion of the Rv0757 gene and PDIM− phenotype from the deletion of the Rv2930 (fadD26) gene, wherein the isolated M. tuberculosis bacterium is a M. tuberculosis MT103 strain or a M. tuberculosis MTBVAC strain, and wherein the unit dose comprises between 3×105 CFU/0.1 ml and 17×106 CFU/0.1 ml of the isolated M. tuberculosis bacterium.
  • 33. The unit dose of claim 32, wherein the isolated M. tuberculosis bacterium is M. tuberculosis MT103.
  • 34. The unit dose of claim 32, wherein the isolated M. tuberculosis bacterium is M. tuberculosis MTBVAC strain.
  • 35. The unit dose of claim 32, wherein the unit dose comprises between 5×105 CFU/0.1 ml and 5×106 CFU/0.1 ml of the isolated M. tuberculosis bacterium.
  • 36. The unit dose of claim 32, wherein the unit comprises 5×105 CFU/0.1 ml of the isolated M. tuberculosis bacterium.
  • 37. The unit dose of claim 32, wherein the unit dose comprises 5×106 CFU/0.1 ml of the isolated M. tuberculosis bacterium.
  • 38. A method of preventing infections caused by M. tuberculosis complex in a non-neonate human at risk of infection with M. tuberculosis complex, the method comprising intradermal administration of the unit dose of claim 32 to the non-neonate human.
  • 39. The method of claim 38, wherein the non-neonate human is a child, adolescent, or adult human.
  • 40. The method of claim 38, wherein the method is for booster vaccination, and the non-neonate human has previously been vaccinated with a Bacille Calmette-Guérin (BCG) vaccine.
Priority Claims (1)
Number Date Country Kind
18382097.6 Feb 2018 EP regional
Continuations (2)
Number Date Country
Parent 18309555 Apr 2023 US
Child 18788724 US
Parent 16971248 Aug 2020 US
Child 18309555 US