LACTIC ACID BACTERIA FOR MODULATING BODY OXYGENATION AND METHODS FOR USING SAME

The invention relates to particular species, strains, and compositions of lactic acid bacteria capable of increasing cellular levels of the hypoxia-inducible factor HIF-1α for the maintenance or enhancement of normoxia in hypoxia-inducing conditions such as, for example, physical exertion, lethargy, chronic fatigue, oxygen deficiency, travel beyond the limits of the earth's atmosphere, oxidative stress of eyeballs and scuba diving, or for the treatment of hypoxia in hypoxia-inducing conditions such as neurodegenerative diseases, pulmonary implications associated with respiratory failure, neonatal hypoxia-ischemia, myocardial ischemia, metabolic disorders, chronic cardiac and renal diseases, reproductive disorders such as pre-eclampsia and endometriosis, exacerbation of postural and kinetic tremors, and cerebral hypoxia.

FIELD OF INVENTION

The invention relates to particular species, strains, and compositions of lactic acid bacteria capable of increasing cellular levels of the hypoxia-inducible factor HIF-1 α for the maintenance or enhancement of normoxia in hypoxia-inducing conditions such as, for example, physical exertion, lethargy, chronic fatigue, oxygen deficiency, travel beyond the limits of the earth's atmosphere, oxidative stress of eyeballs and scuba diving, or for the treatment of hypoxia in hypoxia-inducing conditions such as neurodegenerative diseases, pulmonary implications associated with respiratory failure, neonatal hypoxia-ischemia, myocardial ischemia, metabolic disorders, chronic cardiac and renal diseases, reproductive disorders such as pre-eclampsia and endometriosis, exacerbation of postural and kinetic tremors, and cerebral hypoxia.

BACKGROUND OF THE INVENTION

Oxygen (O2) is an essential nutrient that serves as a key substrate in cellular metabolism and energy production by aerobic organisms. In a variety of physiological and pathological states, organisms experience limited/insufficient O2disponibility, a condition referred to as hypoxia.

O2deprivation creates significant stress in living cells. This condition is related to the inappropriate accumulation of free radicals, which cause further stress on the protein component of cells and the genetic material they contain. To cope with the hypoxic stress condition, cells activate a series of adaptive responses to match 02 supply with metabolic, bioenergetic, and redox demands. In particular, they temporarily arrest the cell cycle, reduce energy consumption, and secrete survival and pro-angiogenic factors. The intestinal mucosa receives between 10% and 35% of the total cardiac output, and the estimated surface area of the gastro-intestinal tract is about 250-300 m2under normal conditions (Lundquist et al., 2016). The gut is characterized by a peculiar oxygenation profile resulting from a combination of different factors, including massive fluctuations in blood perfusion as a result of food ingestion (Matheson et al., 2000). Changes in the amount of blood reaching the gut greatly affect the amount of O2available to the remaining body districts. The gut, therefore, plays a key role in determining the distribution of total O2available to the organism.

In the small intestine, increased oxygen availability sustains intense energy expenditure by highly proliferative stem cells and differentiated post-mitotic cells with high energy demand due to digestive, secretory and absorption processes (Rangel-Huerta et al., 2017; Van Der Schoor et al., 2002). The characteristics of oxygenation and oxygen consumption in the small intestine allow us to hypothesize that their modulation may have a major impact on the redistribution of globally available O2to the body. Under basal physiological conditions, intestinal mucosal epithelial cells are subject to relatively low O2levels, previously described as “physiological hypoxia” (Karhausen et al., 2005). To this condition, intestinal epithelial cells continuously adapt (Shepherd, 1982; Albenberg et al., 2014).

Hypoxia-inducible factors (HIFs) constitute key mediators of intestinal epithelial adaptation to its O2-poor microenvironment (Ramakrishnan et al., 2016). These mediators are responsible for the reduction of oxygen consumption in mitochondria through inhibition of pyruvate to acetyl COA conversion, suppression of mitochondrial biogenesis, and activation of mitochondria autophagy (Goda and Kanai, 2012). The reduction in cellular oxygen consumption associated with HIFs and the subsequent redistribution of oxygen in the peri-cellular microenvironment are supported by evidence produced using PHD inhibitors (Susser et al., 2020). HIFs are heterodimers composed of two subunits termed alpha and beta, respectively, the second of which is constitutively expressed by eukaryotic cells. The HIF-α subunit belongs to the helix-hoop-helix Per-Arnt-Sim (bHLH-PAS) family of basic transcription factors (Schito et al., 2016). Vertebrates possess three subunits α: HIF-1α, HIF-2α and HIF-3α. The N-terminal region of these subunits contains a domain required for DNA binding and heterodimerization (Wu et al., 2015). The HIF-α subunits possess a highly conserved oxygen-dependent degradation (ODD) domain. The ODD domain contains two hydroxylated prolines, in both HIF-1a and HIF-2α (Chan et al., 2005). Hydroxylation of HIF-α leads to proteosomal degradation. The HIF-α subunits are hydroxylated by specific enzymes PHD1 (EGLN2), PHD2 (EGLN1) and PHD3 (EGLN3) belonging to the group of prolyl hydroxylase domain (PHD) enzymes that represent the main oxygen sensors in a cell. Under normoxic conditions, PHDs use O2to hydroxylate HIF-α subunits at the proline level present in the ODD. Hydroxylation allows the binding of the Von Hippel-Lindau oncosuppressor protein (VHL), which acts as an E3 ubiquitin ligase enabling the degradation of HIF-α (Ivan et al., 2001). Under conditions of low oxygen disponibility, PHD enzymes are unable to perform hydroxylation of HIF-α which are stabilized by heterodimerization with an HIF-β subunit (Wang et al., 1995). The generated heterodimer is able to bind genetic elements, termed HIF response elements (HREs) which are present within the promoters of target genes. Consequent to such binding, the target genes are expressed allow the cell to generate an adaptive response to the hypoxic condition (Toescu et al., 2004; Wiener et al., 1996). Although HIF-1a and HIF-2α are closely related and able to activate HRE-dependent expression, both subunits differ in their transactivation domains, implying that they have different gene targets. In particular, scientific evidence has shown that HIF-1a preferentially induces the glycolytic pathway and thus adaptation to energy production in O2deficiency, (Hu et al., 2003). Adaptation to hypoxia associated with HIF activity involves a number of changes in cellular metabolism. Chief among these is the reduction of oxygen consumption by shifting energy production from mitochondrial oxidative phosphorylation to anaerobic glycolysis. Within the intestinal environment, the regulation of HIFs is influenced by multiple factors associated with both cellular metabolism and microbial action (Singhal et al., 2020).

Hypoxic conditions are frequently observed in the presence of a wide variety of pathological conditions, acute and chronic. Hypoxia-associated pathologies include neonatal hypoxia-ischemia, myocardial ischemia, metabolic disorders, chronic cardiac and renal patologies, reproductive disorders such as preeclampsia and endometriosis, exacerbation of postural and kinetic tremors, cerebral hypoxia, and neurodegenerative diseases (Chen et al., 2020; Legros et al., 2010; Nalivaeva et al., 2019; Merelli et al., 2020). Hypoxia assumes relevant importance in pathological conditions resulting from loss of lung surface respiratory function. In this context, the condition of acute respiratory distress caused by infections of the new pandemic coronavirus Sars-COV-2 (Gibson et al., 2020; Ramírez et al., 2020) should be highlighted. In addition, hypoxic conditions are closely related to the onset of altered physiological conditions and pathological manifestations associated with prolonged stay in conditions of low O2availability. In this context, it is incumbent to highlight the pulmonarial, nervous, and muscular impairments associated with activities performed at high altitude. In contrast to reports in the scientifical literature for probiotic microorganisms (Esfandiary et al., 2016; Deepak et al., 2015; Chen et al., 2020; Han et al, 2020), the Applicant surprisingly found that oral administration ofLactobacillus acidophilus, orLactobacillus acidophilusandStreptococcus thermophilusand/orBifidobacterium animalissubsp.lactis, preferably with the addition ofLevilactobacillus brevis(formerly known asLactobacillus brevis),Lactiplantibacillus plantarumsubsp.plantarum(formerly known asLactobacillus plantarum),Lactobacillus helveticus, Lacticaseibacillus paracaseisubsp.paracasei(formerly known asLactobacillus paracaseisubsp.paracasei) is capable of increasing the expression/stabilization of HIF-1α and that particular species, strains, and compositions of lactic acid bacteria are therefore capable of maintaining or enhancing normoxia under hypoxia-inducing conditions such as, e.g., physical exertion, lethargy, chronic fatigue, oxygen deprivation, travel beyond the limits of the earth's atmosphere, oxidative stress of the eyeballs and scuba diving, or for the treatment of hypoxia in conditions involving hypoxia such as neurodegenerative diseases, pulmonary implications associated with respiratory failure, neonatal hypoxia-ischemia, myocardial ischemia, metabolic disorders, chronic cardiac and renal diseases, reproductive disorders such as preeclampsia and endometriosis, exacerbation of postural and kinetic tremors, and cerebral hypoxia.

Compendium of the Invention

An object of the invention is aLactobacillus acidophiluscapable of positively modulating cellular levels of the hypoxia-inducible factor HIF-1α associated with the reduction of cellular oxygen consumption for use in the treatment of hypoxia-inducing conditions such as, for example, physical exertion, lethargy, chronic fatigue, oxygen deficiency, travel beyond the limits of the earth's atmosphere, oxidative stress of eyeballs and scuba diving, or for use in the treatment of hypoxia in conditions involving hypoxia such as neurodegenerative diseases, pulmonary implications associated with respiratory failure, neonatal hypoxia-ischemia, myocardial ischemia, metabolic disorders, chronic cardiac and renal diseases, reproductive disorders such as preeclampsia and endometriosis, exacerbation of postural and kinetic tremors, and cerebral hypoxia.

According to one aspect of the invention, theLactobacillus acidophilusreferred to above is the strain ofLactobacillus acidophilusdeposited by the Applicant under the Budapest Treaty on Sep. 1, 2020 at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having the accession number CNCM I-5567.

A further object of the invention is a composition comprising the aforementionedLactobacillus acidophilusand optionally one or more pharmaceutically acceptable excipients.

According to one aspect of the invention, the composition further comprisesStreptococcus thermophilusand/orBifidobacterium animalissubsp.lactis.

According to a further aspect of the invention,Streptococcus thermophilusis the strain ofStreptococcus thermophilusdeposited by the Applicant under the Budapest Treaty on Sep. 1, 2020 at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having the CNCM accession number I-5570, andBifidobacterium animalissubsp.lactisis the strain ofBifidobacterium animalissubsp.lactisdeposited by the Applicant pursuant to the Budapest Treaty on Sep. 1, 2020 at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having access number CNCM I-5571 and/or the strain ofBifidobacterium animalissubsp.lactisdeposited by the Richidente under the Budapest Treaty on Sep. 1, 2020, at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having accession number CNCM I-5572.

According to a further aspect of the invention, the composition includes from 30% to 50% by weight ofLactobacillus acidophilus, from 25% to 35% by weight ofStreptococcus thermophilus, and from 25% to 35% by weight ofBifidobacterium animalissubsp.lactis, depending on the weight of the composition.

According to a further aspect, theLevilactobacillus brevisstrain is the strain ofLevilactobacillus brevisdeposited by the Applicant under the Budapest Treaty on Sep. 1, 2020 at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having the accession number CNCM I-5566, theLactiplantibacillus plantarumsubsp.plantarumis the strain ofLactiplantibacillus plantarumsubsp.plantarumdeposited by the Applicant under the Budapest Treaty on Sep. 1, 2020 at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having accession number CNCM I-5569, Lacticaseibacillus paracaseisubsp.paracaseiis the strain ofLacticaseibacillus paracaseisubsp.paracaseideposited by the Applicant under the Budapest Treaty on Sep. 1, 2020, at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having accession number CNCM I-5568, andLactobacillus helveticusis the strain ofLactobacillus helveticusdeposited by the Richidente under the Budapest Treaty on Sep. 1, 2020, at the Collection Nationale de Cultures de Microorganismes, Institut Pasteur, 25 rue du Docteur Roux, 75724 Paris Cedex 15, and having accession number CNCM I-5573.

According to a further aspect, the composition includes from 30% to 50% by weightLactobacillus acidophilus, from 1% to 10% by weightStreptococcus thermophilus, from 1% to 20% by weightBifidobacterium animalissubsp.lactis, from 1% to 10% by weightLevilactobacillus brevis(formerly known asLactobacillus brevis), from 1% to 10% by weightLactiplantibacillus plantarumsubsp.plantarum(formerly known asLactobacillus plantarum), from 1% to 10% by weight ofLacticaseibacillus paracaseisubsp.paracasei(formerly known asLactobacillus paracaseisubsp.paracasei), and from 1% to 10% by weight ofLactobacillus helveticus, depending on the weight of the composition.

According to a further aspect, the composition according to the invention is suitable for oral administration, such as in the form of powders, capsules or granules. The composition preferably has a high concentration of bacteria, to the extent of at least 10 billion in the adult and at least 100 million in the infant.

According to a further aspect, the composition according to the invention is suitable for oral administration, such as in the form of powders, capsules, granules or spray, to animals reared and/or maintained in oxygen-deficient conditions, for example, on farms located at relevant heights above sea level.

The used probiotic bacteria may be viable, nonviable, sonicated, tindalized or lyophilized.

Finally, the invention relates to a method for identifyingLactobacillus acidophiluscapable of positively modulating cellular levels of the hypoxia-inducible factor HIF-1α associated with the reduction of cellular oxygen consumption that includes the steps:evaluation, by western blot technique, of cellular levels of HIF-1α in in vitro cellular models suitable for proper physiological representation of the target tissue in the presence and absence of treatment of at 24 hours with bacterial lysate specific to the Lacto-bacillus acidophilusstrain to be evaluated; andevaluation, in the same cellular model, of the extracellular acidification rate (ECAR), oxygen consumption rate (OCR), and the relative glycolysis rate (ECAR/OCR ratio) in the presence and absence of treatment of at 24 hours with bacterial lysate specific to theLactobacillus acidophilusstrain to be evaluated, using the Seahorse XFe96 analyzer (Agilent) according to the manufacturer's instructions or equivalent technique.

DETAILED DESCRIPTION OF THE INVENTION

In Vitro Study

HIF-1α represents a key mediator in the regulation of oxygen homeostasis and preferential induction of the glycolytic pathway and thus adaptation to energy production in O2deficiency resulting in reduced oxygen consumption by shifting energy metabolism to that pathway (Hu et al., 2003).

The inventor conducted in vitro assays on intestinal-derived cellular models in order to evaluate the ability of specific bacterial strains alone or in combinations in modulating HIF-1α accumulation associated with the reduction of cellular oxygen consumption. Obtained results show that, under normoxic conditions, the exposure of Caco-2 cells to bacterial lysates ofL. brevisCNCM I-5566,L. acidophilusCNCM I-5567,L. plantarumCNCM I-5569,L. helveticusCNCM I-5573,L. paracaseiCNCM I-5568,B. lactisCNCM I-5571 andS. thermophilusCNCM I-5570 is associated with a significant increase in intracellular HIF-1α levels compared with the untreated control (FIG.1a).S. thermophilusCNCM I-5570,B. lactisCNCM I-5571 andL. acidophilusCNCM I-5567 were the most effective (˜2.2-fold increase forL. acidophilusCNCM I-5567 and ˜2-fold increase forS. thermophilusCNCM I-5570 andB. lactisCNCM I-5571). In hypoxic conditions, the strains did not induce significant changes compared to untreated cells, except forL. acidophilusCNCM I-5567 whose addition resulted in a significant increase in HIF-1α levels compared to control (FIG.1b). Exposure of Caco-2 cells to combined bacterial extracts at the concentration of 50 and 100 μg/ml was associated with a significant increase in cellular accumulation of HIF-1α under both normoxic and hypoxic conditions (FIGS.2aandb). It is noteworthy that under normoxic conditions, the levels of HIF-1α accumulation recorded for the combined bacterial lysate at the concentration of 100 μg/ml were comparable to those determined at the same concentration for the lysate related toL. acidophilusCNCM strain I-5567 alone. Under hypoxic conditions, already at the concentration of 50 μg/ml, the bacterial lysate related to the combination of probiotic strains induced a cellular accumulation of HIF-1α similar to that recorded forL. acidophilusstrain CNCM I-5567 alone at higher concentrations. Considering that theL. acidophilusstrain CNCM I-5567 represents a quantitatively minority fraction of the bacteria present within the probiotic combination, the observed results suggest that the combined use of the specific probiotic strains tested is characterized by a synergistic effect with respect to the induction of cellular accumulation of HIF-1α.

The influence of lysed bacterial strains on cellular energy metabolism and cellular oxygen consumption was investigated. To this end, levels of L-lactate, a key metabolite of the glycolysis pathway; the extracellular acidification rate of the medium (ECAR), a parameter reflecting glycolysis; and the oxygen consumption rate (OCR) used to determine oxidative phosphorylation were assessed within the culture media. As a result of exposing the Caco-2 cell line to total bacterial lysate for 24 hours, there were significantly lower OCR values attesting to a reduction in cellular oxygen consumption compared to the untreated control (FIG.2c). In contrast, exposure of the cell line to bacterial lysate was associated with a significant increase in Lactate levels, ECAR values and ECAR/OCR ratio attesting to increased glycolysis (FIGS.2a,2band2d).

CONCLUSIONS

The amount of oxygenated blood recalled at the intestinal level conditions the availability of O2in extraintestinal body districts including essential organs such as brain, heart, kidney, and liver.

In the intestine, oxygen homeostasis is largely dependent on HIFs. Probiotic microorganisms have the potential to modulate HIFs and influence the processes regulated by them. Strains belonging to the bacterial speciesL. paracasei, L. acidophilus, L. crispatus, L. rhamnosus, andB. longumare able to inhibit, in vitro, the expression of HIF-1α in various cellular models (Han et al., 2020; Esfandiary et al., 2016; Deepak et al., 2015; Chen et al., 2020). Contrary to reports in the literature, the inventor's results showed, surprisingly, that the tested probiotic microorganisms are able to positively modulate the accumulation of HIF-1α. This contrasting effect, finds an explanation in the fact that the regulation of HIF-1α reflects the involvement of different molecular mechanisms. In addition, the beneficial effect produced by probiotics depends on the specific physiological state of host cells (McFarland et al., 2018). The increased accumulation of HIF-1α induced by the tested bacterial species is associated with a significant reduction of oxygen consumption in intestinal cells and the induction of anaerobic metabolism, which allows their survival under conditions of scarcity of this gas. The oxygen sparing induced by the tested bacteria could modulate the consumption of such gas in the intestine. The amount of O2not consumed in that body district could become available to other essential organs and tissues.

Materials and Methods

Cell Cultures and Treatments

The human colon adenocarcinoma cell line (Caco-2) was cultured in DMEM (Dulbecco's Modified Eagle's Medium) medium containing 10% (v/v) fetal bovine serum, 1% nonessential amino acids, 1 mM sodium pyruvate, 2 mM glutamine, 100 U/ml penicillin and 100 μg/ml streptomycin and incubated in a humidified atmosphere with 5% CO2at 37° C. After reaching 80% confluence, the cells were detached and plated in a multiwell plate of 6 at the concentration of 6×104cells/cm2. Cell growth was monitored by light microscopy. For assessment of cellular HIF-1α levels of extracellular acidification rate and oxygen consumption rate, cells differentiated at 14 days post-confluence were pretreated with or without the indicated concentration of probiotic for min and then incubated in normoxia under standard culture conditions, (˜21% O2) or in hypoxia using a “hypoxia incubation chamber” (1% O2) for 24 hr.

Preparation of the Soluble Fraction of Bacterial Lysates

The soluble fraction of bacterial lysates was prepared as follows: each sample was washed three times (8,600×g for 20 min at 4° C.) and resuspended in phosphate buffered saline (PBS). The bacterial suspension was sonicated for 30 minutes, alternating 10 seconds of sonication and 10 seconds of pause, and centrifuged at 17.949×g for 20 minutes at 4° C. The supernatant was filtered through a 0.22 μm filter so as to remove any remaining intact bacteria, and the protein concentration was determined. For tests on individual bacterial strains, the concentration of the soluble fraction of the bacterial lysate was determined to be 100 μg/ml. The assays concerning probiotic strain combinations, were performed with increasing concentrations of total bacterial lysate soluble fraction of 10, 50 and 100 μg/ml, respectively. The assays performed to evaluate the action of the combination of strains was carried out on a probiotic formulation in which the percentage of bacterial cells of each individual strain to total bacterial cells in the compound was as follows: 35.46%L. brevisCNCM I-5566, 1.42%L. acidophilusCNCM I-5567, 5.32%L. plantarumCNCM I-5569, 0.71%L. helveticusCNCM I-5573, 2.13%L. paracaseiCNCM I-5568, 17.73%B. lactisCNCM I-5571, 1.77%B. lactisCNCM I-5572 and 35.46%S. thermophilusCNCM I-5570. The samples thus prepared were frozen at −80° C. until use. Untreated cells were considered as controls.

Western Blot

HIF-1α expression was assessed by Western blotting. Cells were lysed on ice using RIPA buffer containing protease inhibitors for 30 min on ice. After cell lysis, samples were centrifuged at 17,949×g for min at a temperature of 4° C. The supernatant was recovered and the total protein assay was performed. Sample buffer and mercaptoethanol was added to a volume of supernatant equivalent to g of protein, and samples were boiled for 5 min and separated by sodium dodecyl sulfate (SDS)-polyacrylamide 10% gel electrophoresis (SDS-PAGE). Transfer of samples onto nitrocellulose membrane (0.45 μm) was carried out at constant 70 volts for 1 h at 4° C., and the nitrocellulose filter was incubated at room temperature for 1 h with a specific site blocking solution and then incubated overnight at 4° C. with monoclonal anti-HIF-1α or anti-β-actin antibody. After incubation with the secondary antibody, conjugated with horseradish peroxidase (HRP), the immunoreactive bands were visualized by chemiluminescence. Densitometric analysis of the bands corresponding to HIF-1α was then performed, and the values obtained were normalized to those of β-actin.

L-lactate levels in cell culture supernatants were assayed using the L-lactate assay kit (Abcam, Cambridge, UK) according to the manufacturer's instructions. Supernatants were deproteinized with a 10-kDa NMWCO centrifugal filtration unit (Amicon, Millipore), and the filtrate was added to reaction wells. Absorbance was measured by spectrophotometric reading at 570 nm.

Metabolic Studies

Cells treated as described above were evaluated for extracellular acidification rate (ECAR) and oxygen consumption rate (OCR) to calculate the rate of glycolysis (ECAR/OCR) using the Seahorse XFe96 analyzer (Agilent) following the manufacturer's instructions. Briefly, on the day of the test, the medium was changed to Seahorse XF DMEM Medium pH7.4 supplemented with glucose (10 mmol/L), pyruvate (1 mmol/L) and glutamine (2 mmol/L) (Agilent), and the cells were allowed to equilibrate in a non-CO2incubator for 1 h; OCR and ECAR were then measured. XFp Mito Stress Test Kit was used to test mitochondrial function. Injection of oligomycin (1 μM), carbonyl cyanide-4 (trifluoromethoxy) phenylhydrazone (FCCP, 1 μM), and the mixture of rotenone and antimycin A (1 μM) allowed the determination of key bioenergetic parameters: basal respiration, ATP production-related respiration (ATP production), maximal respiration, reserve respiratory capacity, nonmitochondrial respiration, proton leakage, and coupling efficiency.

ANOVA test followed by Dunnett's or Tuckey post hoc tests was used to check for statistically significant differences between the different conditions tested while, in the case of two groups, comparisons between mean values were made by unpaired Student's t test. A p value≤0.05 was considered statistically significant. Analyses were performed using R 4.0.3 statistical software.

In Vivo Study

Reduced oxygen supply to the brain plays a key role in neurodegeneration during the aging process (Ogunshola and Antoniou, 2009). Pathological processes such as oxidative stress, impaired oxygen or glucose supply, and disruption of iron homeostasis are common in neurodegenerative diseases (Correia and Moreira, 2010; Gironi et al., 2011; Benarroch, 2009). Reduced brain levels of HIF-1α, associated with decreased expression of GLUT1 and GLUT2 receptors responsible for glucose uptake, have been previously demonstrated in models of Alzheimer's disease (AD). The inventor conducted in vivo assays in order to evaluate the ability of a specific bacterial combination in modulating HIF-1α accumulation in brain tissue of 3×Tg-AD mice. This reliable model of human AD shows both plaque and tangle pathology, with intracellular AB immunoreactivity detectable at three months of age and hyperphosphorylation of tau protein occurring between 12 and 15 months of age (Oddo et al., 2003). The characteristics of the experimental design, as well as, the preparation of brain extracts were in line with what was previously reported in 2018 by Bonfili et al. (Bonfili et al., 2018). Fortyeight 3×Tg-AD guinea pigs, eight weeks old, were divided into 2 groups. The first group (n=24) was treated with a specific probiotic formulation containingStreptococcus thermophilusCNCM I-5570,Bifidobacterium animalissubsp.lactisCNCM I-5571,Bifidobacterium animalissubsp.lactisCNCM I-5572,Lactobacillus acidophilusCNCM I-5567,Lactobacillus helveticusCNCM I-5573, Lacticaseibacillus paracaseisubsp.paracaseiCNCM I-5568, Lactipantibacillus plantarumsubsp.plantarumCNCM I-5569 andLactobacillus brevisCNCM I-5566 while the other (n=24), untreated, was used as a control. Simultaneously, 48 wild-type (wt) mice of the same age were also divided into 2 groups of equal numbers, only one of which was treated with the same probiotic formulation. The dosage (200 billion bacteria/kg/day) was determined using body surface area normalization as previously reported in the literature (Crawford et al., 1950). Mice were sacrificed for biochemical analysis at 24 and 56 weeks of age (16 and 48 weeks from the start of treatment), and brains were stored at −80° C. until brain homogenates were produced. ANOVA followed by Bonferroni's test was used to test for statistically significant differences in HIF-1α expression levels. A p value≤0.05 was considered statistically significant. The level of HIF-1α subunit in brain homogenates was analyzed by Western blotting assay as previously described (Bonfili et al., 2018). The results obtained showed that untreated 3×Tg-AD mice had significantly lower brain levels of HIF-1α than wt mice of the same age. Surprisingly, administration of a probiotic formulation in 3×Tg-AD mice was associated with a significant increase in brain levels of HIF-1α. Unexpectedly, treatment with the probiotic restored HIF-1α expression to the levels recorded for wt mice of equal age (FIG.3). The increased brain levels of HIF-1α observed suggest that administration of the specific probiotic formulation tested could improve oxygen homeostasis and glucose metabolism in the brain constituting a viable therapeutic approach for the treatment of neurodegenerative diseases.

Studies Performed on Humans

First Study on Humans

In this study, the effect of taking a specific probiotic formulation on respiratory, cardiac, and metabolic parameters in subjects practicing endurance sports was evaluated. For this purpose, 4 male Triathlon praticants subjects (Age: mean±DS, 37±5 years; Weight: mean±DS 70±3 kg) were recruited. Two sets of trials were carried out, the first of which denoted “PRE” involved carrying out the protocol in the absence of intake of specific probiotic formulation. In the second set of trials, called “POST,” the same subjects repeated the test after intake of a bacterial composition consisting ofStreptococcus thermophilusCNCM I-5570,Bifidobacterium animalissubsp.lactisCNCM I-5571,Bifidobacterium animalissubsp.lactisCNCM I-5572,Lactobacillus acidophilusCNCM I-5567,Lactobacillus helveticusCNCM I-5573, Lacticaseibacillus paracaseisubsp.paracaseiCNCM I-5568, Lactipantibacillus plantarumsubsp.plantarumCNCM I-5569 andLactobacillus brevisCNCM I-5566. The amount of probiotics taken consisted of the ingestion of about 400 billion bacterial cells in a single dose. Subjects were asked to consume their last meal with dinner on the day before the tests and to appear fasting at their assigned time, allowing water intake only; in the “POST” test sets, they were asked to take the probiotic formulation no earlier than 5 hours after the last meal and at least 5 hours before the time of the test. The tests were conducted midweek to minimize the impact of physical activity during the weekend. Each subject repeated the two sets of tests on the same day and at the same time. The tests were performed on a Panatta Treadmill model T-190 (Panatta, Italy) with a fixed belt incline of 1%. After subjects were made to wear the metabolimeter mask, they were allowed to perform a 5′ warm-up at free intensity, but lower than the test intensity. Successively, without interruption the intentionality was increased to a threshold value for another 10′. This value was chosen using individual subjects' knowledge of their own anaerobic threshold intensity and represented an appropriate exercise intensity for running a total distance of 20 km. Measurements of the average heart rate over the last 5 minutes of exercise and the amount of oxygen that the body is able to extract and then use in the unit of time for muscle contraction (VO2) were acquired using Fitmate PRO equipment (COSMED, Italy) interfaced with a heart rate monitor band (POLAR, Italy). Blood lactate concentration was determined by capillary sampling from the earlobe performed at the end of the threshold intensity step. With respect to the parameters considered, the presence of significant differences between the PRE and POST test groups was assessed by Student's t test for paired data. A p value≤0.05 was considered statistically significant. Lactate represents the end product of the glycolithium cycle when it is carried out in oxygen deficiency so its concentration reflects the level of anaerobic metabolism. Heart rate and VO2constitute additional parameters that can give indications of the level of aerobic metabolism as a reduction in these parameters indicates an improvement in aerobic metabolism and thus greater oxygen availability. In general, the reduction in heart rate, VO2and blood lactate concentration suggest an improvement in the efficiency of aerobic metabolism associated with the intake of the probiotic formulation (FIG.4).

These results are consistent with the hypothesis that the positive modulation of HIF-1α, induced by the action of specific probiotic strains in the intestine, would allow a reduction in O2consumption in that district. The oxygen sparing induced by probiotic intake would cause this gas to be redistributed by becoming more available in the blood circulation and consequently to other body districts.

Second Study on Humans

Hypoxia is a common condition in many disease states that takes on particular relevance in conditions associated with acute lung injury (Lee et al., 2019). The purpose of the present work was to investigate the baseline action performed by bacterial strains in alleviating respiratory conditions in subjects with pulmonary implications associated with Sars-COV-2 infections. In addition, the earliness with which this beneficial effect appear evident was evaluated. To this aim, responses of two groups of patients was examined, one group was treated with the best available therapy (BAT), while the other was additionally supplemented with oral bacteriotherapy (BAT+OB). The effect of probiotic intake was evaluated by comparing the blood oxygenation parameters partial pressure of oxygen (pO2), fraction of inspired oxygen (FiO2), oxygenated hemoglobin (O2Hb), pO2/FiO2ratio, and oxygen-saturated hemoglobin (SaO2) of the two groups at the beginning of treatment and in the following twenty-four hours. The amount of oxygen delivered (l/min) was additionally measured. The main characteristics of both groups of patients are summarized in Table 1.

With the exception of sex, the two groups determined by the administration of the probiotic formulation were homogeneous for all clinical considered variables including drug therapies for treatment of SARS-COV-2 infections, blood oxygenation parameters and amount of oxygen administered (median; IQR BAT 4; 1-6 l/min; BAT+OB 1.5; 1-6 l/min, p=0.31). Twenty-four hours after the first probiotic dose, the BAT+OB group showed significantly higher values of the pO2/FiO2ratio and pO2than the BAT group while an opposite situation was observed for FiO2values (FIGS.5a-c). Analysis of O2Hb and SaO2levels produced results in line with those previously described for the pO2and pO2/FiO2ratio (FIGS.5eand5f). Overall results showed that after 24 hours from the start of treatments, the group administered with the probiotic formulation had better blood oxygenation levels than the group taking only the standard therapy, although the BAT group experienced a significantly higher increase in the amount of oxygen delivered over time (FIG.5d).

The improvement in blood oxygenation parameters observed in the BAT+OB group are consistent with the hypothesis that, at the gut level, the positive modulation of HIF-1α induced by the action of specific probiotic strains would allow a reduction in O2consumption which would be redistributed by becoming more available at the level of the bloodstream.

Patients and Methods

Study Design, Population of Subjects, Data Collection and Treatment

This study was performed on SARS-COV-2 infected adult patients (>18 years), supported with oxygen therapy sumministrated via Venturi mask under spontaneous breathing regimen. The diagnosis of SARS-COV-2 infection was defined by a positive oropharyngeal and nasopharyngeal swab performed in duplicate for SARS-COV-2 E and S gene by reverse transcriptase polymerase chain reaction (RT-PCR). Patients included in the study were housed in two different wards devoted to the management of COVID-19: in the first ward, only BAT was administered as suggested by the Società Italiana di Malattie Infettive e Tropicali (SIMIT) (Italian Society of Infectious and Tropical Diseases) and Italian Medicine Agency (AIFA) interim guidelines, comprising Dexamethasone (6 mg daily for 10 days) plus low molecular weight heparins (prophylactic dosage)+/−azithromycin (500 mg daily); Remdesevir, as per AIFA guidelines. In the second ward, BAT was combined with the administration of oral bacteriotherapy consisting of a total of 2,400 billion bacteria per day comprisingS. thermophilusCNCM I-5570,B. lactisCNCM I-5571,B. lactisCNCM I-5572,L. acidophilusCNCM I-5567,L. helveticusCNCM I-5573,L. paracaseiCNCM I-5568,L. plantarumCNCM I-5569, andL. brevisCNCM I-5566 strains. Considered variables included 1) medical history data, 2) past medical history (comorbidities), 3) current medical history, treatment, and laboratory data. Arterial blood gas analysis (ABG test) was performed using blood taken from the radial artery 24 hours after the start of treatments.

Statistical Analysis

Categorical variables including sex, antiviral drug therapy, and antibiotic administration were compared using the χ2test with Yates continuity correction to account for the limited sample size and shown as absolute frequencies and percentages. The two-sided Mann-Whitney U-test was used for all continuous variables including respiratory variables (pO2, FiO2, pO2/FiO2Change in oxygens supplied compared to treatment onset, O2Hb, SaO2), biochemical variables (blood glucose, lactates, hematocrit) and demographic and clinical variables (age, BMI, ALT, AST, Charlson Index) in order to determine statistically significant differences between groups at each considered time point while, for each group, the Wilcoxon test was used to assess significant differences between consecutive time points. In all cases a p-value≤0.05 was considered statistically significant.

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