Patent Description:
Pleuromutilin, a compound of formula
<CHM>
is a naturally occurring antibiotic, produced e.g. by the basidiomycetes Pleurotus mutilus and P. passeckerianus, see e.g. <NPL>.

A number of further Pleuromutilins having the principle ring structure of Pleuromutilin and being substituted at the primary hydroxy group have been developed, e.g. as antibacterials. Due to their pronounced antibacterial activity, a group of Pleuromutilin derivatives, amino-hydroxy-substituted cyclohexylsulfanylacetylmutilins, as disclosed in <CIT>, have been found to be of particular interest. As described in <CIT><NUM>-O-{[(<NUM>-Amino-<NUM>-hydroxy-cyclohexyl)-sulfanyl]-acetyl}-mutilins are particularly useful compounds because of their activity against Gram-positive and Gram-negative bacteria.

Pharmaceutical active compounds derived from Pleuromutilin (semi synthetic compounds) are inhibitors of ribosomal protein synthesis in bacteria. Representatives of semisynthetic Pleuromutilins for human use are Retapamulin (approved as AltargoP®, AltabaxP®), a topical agent approved for short term treatment of impetigo and infected small lacerations, abrasions or sutured wounds, and Lefamulin (approved as Xenleta®) for the treatment of adults with community-acquired bacterial pneumonia (CABP). Tiamulin (Denagard®) and Valnemulin (Econor®) are two other semi-synthetic Pleuromutilin derivatives which have been used systemically as antibiotics in veterinary medicine for many years. <CHM>
<CHM>.

Approved semisynthetic compounds derived from Pleuromutilin have shown excellent activity against bacterial organisms which include inter alia Streptococcus pneumoniae, Haemophilus influenzae, Staphylococcus aureus (including MRSA), Moraxella catarrhalis, Legionella pneumophila, Chlamydophila pneumoniae and Mycoplasma pneumoniae.

Viral diseases are one of the leading causes of morbidity and mortality in the world. Respiratory viruses such as influenza, respiratory syncytial virus, certain adenoviruses, rhinoviruses and corona viruses and in particular the newly emerged severe acute respiratory syndrome coronavirus <NUM> (SARS-CoV-<NUM>; COVID-<NUM>) have a significant impact on public health.

In <NPL>, for the first time the antiviral activity of Pleuromutilins was described with antiviral activity of Pleuromutilin itself for an influenza A virus strain (PR8) at a concentration of <NUM>/mL. In contrast, Pleuromutilin did not show antiviral activity for polio virus in this study.

Furthermore, in <NPL>, the antiviral activity of Pleuromutilin against both, DNA and RNA viruses, in particular herpes simplex type <NUM> (HSV-<NUM>) virus at a test compound concentration that conferred a <NUM>% protection of the cytopathic effect induced by HSV-<NUM> (CPE50) of <NUM> (<NUM>µg/mL) and activity against vesicular stomatitis virus (VSV) is described.

In <CIT> the use of Tiamulin as an antiviral agent is claimed, with effect of Tiamulin on influenza A virus, porcine reproductive and respiratory syndrome virus (PRRSV) type <NUM> and <NUM> in a viral up-take assay <NUM> hours post inoculation with the virus at Tiamulin concentrations of <NUM>-<NUM>µg/mL compared to Valnemulin and the effect of Tiamulin on endosomal pH exemplified. Valnemulin did not exhibit antiviral activity and it was stated that other Pleuromutilin antibiotics have not been found to have an effect on viruses.

Alteration of the endosomal or lysosomal pH by Tiamulin and associated prevention of fusion of the viral membrane with endo- and lysosomes, which is a pre-requisite for viral entry, was described as potential mode-of-action.

<CIT> and <CIT> both disclose further Pleuromutilin derivatives and generally mention their use in antiviral drugs, without, however, disclosing any actual proof for an antiviral action.

Certain statements about potential antiviral and anti-inflammatory effects of Lefamulin were made in the "<NPL>, downloaded June <NUM>, <NUM> as well as in a press release of May <NUM>, <NUM> (https://investors. com/news-releases/news-release-details/nabriva-therapeutics-reports-first-quarter-<NUM>-financial), downloaded May <NUM>, <NUM>.

Surprisingly, it was now found that the Pleuromutilin derivatives disclosed in <CIT> are effective against viruses and, thus, effective against diseases mediated by viruses.

Therefore, in a first aspect the present invention relates to a compound as defined in claims <NUM> to <NUM>, in particular Lefamulin, or a pharmaceutically acceptable salt, or solvate thereof, for the specific use in the treatment or prevention of a disease mediated by a virus.

In a further aspect, the present invention relates to a method of treatment or prevention of a disease mediated by a virus, comprising administering a compound as defined in any of claims <NUM> to <NUM>, in particular Lefamulin, or a pharmaceutically acceptable salt, or solvate thereof to a subject in need of such treatment.

Lefamulin is the INN for a compound of generic formula (I), more particular, Lefamulin is a compound of formula (VII)
<CHM>
i.e. <NUM>-O-{[(<NUM>R, <NUM>R, <NUM>R)-<NUM>-amino-<NUM>-hydroxy-cyclohexylsulfanyl]-acetyl}-mutilin (also known as "BC-<NUM>").

In the following, the term "Lefamulin", when generally used without additional explanation, is intended to encompass both Lefamulin in free base form, as well as its salts and solvates.

Lefamulin has been developed for systemic use to treat serious bacterial infections in humans and was approved for medical use in the United States in <NUM> to treat adults with community-acquired bacterial pneumonia (CABP).

The present invention refers to the treatment and prevention of a disease mediated by viruses, e.g. a viral disease or viral infection.

The results of the experiments show that besides its antibacterial activity, Lefamulin is also actively reducing the cytopathic effect mediated by different viruses. This antiviral effect was particularly shown for such viruses that are characterized in that they are positive- or negative sense single-stranded RNA viruses. Antiviral activity was shown for both enveloped and non-enveloped viruses, in particular several enveloped positive- or negative sense single-stranded RNA viruses (such as Coronaviridae, Paramyxoviridae, Orthomyxoviridae, and Flaviviridae). Moreover, some of the investigated viruses, including measles virus are known for a transmission involving the respiratory route, in particular airborne transmission. Corona virus and Respiratory Syncytial Virus also cause infections of the respiratory tract in humans.

In a preferred embodiment of the present invention, the virus is a positive- or negative-sense single-stranded RNA virus,
preferably the virus is selected from the group consisting of.

In an other embodiment, the disease is an airborne disease. An airborne disease is mediated by a virus transmitted by the air.

Viral infections can affect various organs. In a preferred embodiment of the present invention, the disease is a respiratory disease, including upper and lower respiratory infections, in particular lower respiratory infections.

In particular, the disease is an acute respiratory syndrome, such as Influenza, Severe Acute Respiratory Syndrome (SARS), Middle East Respiratory Syndrome (MERS) or COVID-<NUM>.

In a further embodiment of the present invention the disease is mediated by a virus selected from the group consisting of viruses of the virus families Coronaviridae, in particular a corona virus such as SARS-CoV, SARS-CoV2, MERS-CoV or HCoV-229E, Orthomyxoviridae, in particular an Influenza virus such as Influenza A and B viruses, Paramyxoviridae in particular Respiratory Syncytial Virus and Adenoviridae, in particular Adenovirus.

In an embodiment, the virus is a corona virus, in particular selected from the group consisting of SARS-CoV, SARS-CoV2, MERS-CoV, and HCoV-229E as well as mutations thereof. Such corona viruses are known to cause (severe) acute respiratory syndromes, such as SARS, MERS or COVID-<NUM>.

Treating, treatment or to treat as understood herein includes on one hand the complete curing, curation or to cure a condition (the disease mediated by a virus) such that it comes to its end and on the other hand also ameliorating, amelioration or to ameliorate a condition such that its symptoms are reduced at least partially or individually.

Treatment typically includes administering a compound as used according to the present invention to a subject in need thereof, i.e. a subject being diagnosed to have a disease mediated by a virus.

Preventing, prevention, or to prevent includes administering a compound before a condition is diagnosed or before onset of (all) disease symptoms of the condition.

Prevention of diseases mediated by viruses includes administering the compounds before onset of disease symptoms. Prevention may be considered after a subject has been infected with a virus but has not shown any symptoms, or wherein a subject has been exposed and/or is prone to exposition to a virus.

The appropriate dosage of the compound to be administered according to the present invention, in particular Lefamulin, will, of course, vary depending upon, for example, the individual host, the mode of administration and the nature and severity of the conditions being treated. However, in general, for satisfactory results in larger mammals, for example humans, an indicated daily dosage is in the range from about <NUM> to <NUM> of a compound used according to the present invention conveniently administered, for example, in divided doses up to four times a day.

The compound used according to the present invention may be administered by any conventional route, for example enterally, e.g. including nasal, buccal, rectal, oral administration; parenterally, e.g. including intravenous, intramuscular, subcutaneous administration; or topically, e.g. including pulmonary, epicutaneous, intranasal, intratracheal administration, e.g. in form of coated or uncoated tablets, capsules, injectable solutions or suspensions, e.g. in the form of ampoules, vials, in the form of ointments, creams, gels, pastes, inhaler powder, foams, tinctures, lip sticks, drops, sprays, or in the form of suppositories, e.g. in analogous manner to the antibiotic agent tobramycin or macrolides, such as erythromycins, e.g. clarithromycin or azithromycin.

Preferably, the compound used according to the present invention is administered via inhalation, via intravenous or subcutaneous injection, or orally.

Preferred pharmaceutical compositions of Lefamulin for injection are disclosed in <CIT>.

The compound used according to the present invention, in particular Lefamulin, may be administered in the form of a pharmaceutically acceptable salt, e.g. an acid addition salt, or in free form, optionally in the form of a solvate.

In one embodiment, the compound is in the form of a salt and/or a solvate.

A salt of a compound used according to the present invention includes an acid addition salt.

Pharmaceutically acceptable acid addition salts include salts of a compound used according to the present invention with an acid, e.g. hydrogen fumaric acid, fumaric acid, tartaric acid, ethane-<NUM>,<NUM>-disulphonic acid, maleic acid, naphthalin-<NUM>,<NUM>-sulphonic acid, acetic acid, malic acid, lactic acid, i.e. L-lactic acid, succinic acid, salicylic acid, azelaic acid, <NUM>-[(<NUM>,<NUM>-dichlorophenyl)amino]benzene acetic acid, hydrochloric acid, deuterochloric acid, preferably hydrochloric acid, acetic acid, L-lactic acid, and maleic acid.

Of these, in the case of Lefamulin, the acetate salt of Lefamulin is especially preferred.

Preferred crystalline forms of Lefamulin as well as crystalline salt forms of Lefamulin are disclosed in <CIT>. Of these, the acetate salt of Lefamulin in crystalline Form B as disclosed in <CIT> is especially preferred.

The present invention also provides the Lefamulin in its form as acid addition salt with itaconic acid, in particular Lefamulin itaconate. Lefamulin itaconate is disclosed herein as a new compound (Example <NUM>). Itaconic acid can be deprotonated to the anions hydrogen itaconate and itaconate. The acid addition salt comprising Lefamulin as cation and an anion derived from itaconic acid is expected to be useful as antiviral agent.

The compound used according to the present invention, in particular Lefamulin, may be used for the pharmaceutical treatment contemplated herein alone or in combination with one or more other pharmaceutically active agents. Such other pharmaceutically active agents include e.g. other antiviral agents. Such other antiviral agents may preferably be selected from the group consisting of nucleoside and nucleotide analogues and RNA polymerase inhibitors, e.g. Remdesivir or Ribavirin, viral protease inhibitors such as Lopinavir or Ritonavir, viral neuraminidase inhibitors, such as Oseltamivir, and other agents used in antiviral therapy such as Hydroxychloroquine, interferons (interferon alfa and/or beta), or other broad-spectrum antiviral agents.

Combinations include fixed combinations, in which two or more pharmaceutically active agents are in the same formulation; kits, in which two or more pharmaceutically active agents in separate formulations are sold in the same package, e.g. with instruction for coadministration; and free combinations in which the pharmaceutically active agents are packaged separately, but instruction for simultaneous or sequential administration are given.

A pharmaceutical composition comprising a compound used according to the present invention, in particular Lefamulin may in addition comprise at least one pharmaceutically acceptable excipient, e.g. carrier or diluent, e.g. including fillers, binders, disintegrators, flow conditioners, lubricants, sugars and sweeteners, fragrances, preservatives, stabilizers, wetting agents and/or emulsifiers, solubilizers, salts for regulating osmotic pressure and/or buffers.

Such pharmaceutical compositions may be manufactured according, e.g. analogously, to a method as conventional, e.g. by mixing, granulating, coating, dissolving, spray drying, or lyophilizing processes. Unit dosage form may contain, for example, from about <NUM> to about <NUM>, such as <NUM> to about <NUM>.

A subject in need of a treatment as contemplated by the present invention may be any living subject suffering from a disease mediated by a virus. Especially, the subject may be a human or an animal.

Herein, including the examples, the following abbreviations are used:.

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability following alpha coronavirus 229E (HCoV-229E or CoV229E) in MRC-<NUM> cells <NUM> days post infections with the virus by various concentrations of Lefamulin (BC-<NUM>).

Methodology: MRC-<NUM> cells were seeded in <NUM>-well flat-bottom tissue culture plates (at a density of <NUM> x <NUM><NUM> cells per well) and allowed to adhere overnight. Thereafter, diluted test compounds (Lefamulin as acetate, Tiamulin as fumarate) dissolved in DMSO were added to the plate and incubated for <NUM> hours prior to addition of the virus. The virus was added diluted to a pre-determined titer to yield <NUM>-<NUM>% cell killing at <NUM> days post-infection (MOI of <NUM>).

Following incubation at <NUM> and at <NUM>% CO<NUM> for <NUM> days, cell viability was measured by XTT tetrazolium dye staining. The optical density of the cell culture plate was determined spectrophotometrically at <NUM> and <NUM>. Percent reduction of the virus-infected cells and the percent cell viability of uninfected drug control wells were calculated to determine the effective concentration at which <NUM>% of cytopathic effect was inhibited (EC<NUM>) and the cytotoxic concentration (TC<NUM>) using four parameter curve fit analysis. The antiviral compound Remdesivir served as positive control.

Surprisingly, Lefamulin reduced the viral CPE by <NUM>% at a concentration of <NUM>, which is a concentration that had no cytotoxic effect on the viability of the cell control. The calculated EC<NUM> was <NUM>, at which <NUM>% of the viral cytopathic effect was inhibited. At the Lefamulin concentration of <NUM>, Lefamulin displayed a cytotoxic effect; the calculated TC<NUM> was <NUM>. The ratio of EC<NUM> and TC<NUM>, known also as therapeutic index, was <NUM>.

In contrast, Tiamulin at a concentration of <NUM> reduced the viral CPE only by <NUM>% and no cytotoxic effect was observed. At the next higher test concentration of <NUM> the CPE was reduced by <NUM>% and a cytotoxic effect was observed. The calculated EC<NUM> was <NUM> and the calculated TC<NUM> was <NUM>. The therapeutic index of Tiamulin was <NUM> and surprisingly much lower than that of Lefamulin.

The antiviral compound Remdesivir was developed as a treatment for Ebola virus, and also is known to have antiviral activity against corona viruses (clinical investigation is ongoing).

Thus, Remdesivir served as positive control herein. Remdesivir showed an EC<NUM> of <NUM>, a TC<NUM> of > <NUM> and a therapeutic index of > <NUM>.

The results are graphically displayed in <FIG> (Lefamulin), <NUM> (Tiamulin) and <NUM> (Remdesivir) (VC. reduction in viral CPE, CC. Cell Control).

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability following alpha coronavirus 229E (HCoV-229E or CoV229E) in MRC-<NUM> cells for Lefamulin at various treatment conditions.

Method: The assay was performed in analogy to Example <NUM> above with the following differences regarding the test candidate. Lefamulin (as acetate) was evaluated using different treatment conditions of <NUM>, <NUM> or <NUM> incubation prior to virus addition and addition <NUM> after infection For this particular set of experiments, coronavirus was diluted <NUM>:<NUM> in assay medium and added at <NUM>µL/well to achieve approximately <NUM>% cell killing in the untreated virus control wells (MOI of <NUM>).

The antiviral efficacy and cellular toxicity data are summarized in the table below. Lefamulin showed a time-dependent effect on the inhibition of the virus-induced cytopathic effects (CPE). In the treatment setting after viral exposure (<NUM> post-infection) a dose-dependent effect was observed. At a concentration of <NUM> the viral CPE was reduced by <NUM> % (data not shown in detail).

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability following human respiratory syncytial virus (strain RSVA2) replication in HEp2 cells <NUM> days post infections with the virus by various concentrations of Lefamulin (BC-<NUM>).

Methodology: HEp2 cells were seeded in <NUM>-well flat-bottom tissue culture plates (at a density of <NUM> x <NUM><NUM> cells per well) and allowed to adhere overnight. Thereafter, diluted test compounds (Lefamulin as acetate, Tiamulin as fumarate) in DMSO were added to the plate and incubated for <NUM> hours prior to addition of the virus. The virus was added diluted to a pre-determined titer to yield <NUM>-<NUM>% cell killing at <NUM> days post-infection (MOI of <NUM>).

Following incubation at <NUM> and at <NUM>% CO<NUM> for <NUM> days, cell viability was measured by XTT tetrazolium dye staining. The optical density of the cell culture plate was determined spectrophotometrically at <NUM> and <NUM>. Percent reduction of the virus-infected cells and the percent cell viability of uninfected drug control wells were calculated to determine the effective concentration at which <NUM>% of cytopathic effect was inhibited (EC<NUM>) and the cytotoxic concentration (TC<NUM>) using four parameter curve fit analysis. The antiviral compound TMC353121 (RSV fusion inhibitor) served as positive control.

Surprisingly, Lefamulin reduced the viral cytopathic effect (CPE) by <NUM>% and <NUM>% at concentrations of <NUM> and <NUM>, respectively, which are concentrations that had no cytotoxic effect on the viability of the cell control. The calculated EC<NUM> was <NUM>, at which <NUM>% of the viral CPE was inhibited. At the Lefamulin concentration of <NUM>, Lefamulin displayed a cytotoxic effect; the calculated TC<NUM> was <NUM>. The ratio of EC<NUM> and TC<NUM>, known also as therapeutic index, was <NUM>.

In contrast, Tiamulin at a concentration of <NUM> reduced the viral CPE only by <NUM>% and a cytotoxic effect (<NUM>% viability) was observed at this concentration. At the next higher test concentration of <NUM> the viral CPE was reduced by <NUM>% and at the cytotoxic effect was more pronounced (<NUM>% viability). The calculated EC<NUM> was with ><NUM> above the calculated TC<NUM> of <NUM>. The therapeutic index of Tiamulin therefore could not be calculated. Surprisingly, the antiviral activity and the therapeutic index was much higher for Lefamulin than for Tiamulin.

The antiviral compound TMC353121 was developed as a specific respiratory syncytial virus fusion inhibitor (clinical investigation is ongoing). Thus, TMC353121 served as positive control herein. TMC353121 showed an EC<NUM> of <NUM>, a TC<NUM> of > <NUM> and a therapeutic index of > <NUM>.

The results are graphically displayed in <FIG> (Lefamulin), <NUM> (Tiamulin) and <NUM> (TMC353121) (VC. Reduction in viral CPE, CC. Cell Control).

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability following human respiratory syncytial virus (strain RSVA2) replication in HEp2 cells changing the multiplicity of infection (MOI).

Methodology: The assay was performed in analogy to Example <NUM> above with the following differences regarding the test. The virus was added diluted to a pre-determined titer to yield <NUM>-<NUM>% cell killing at <NUM> days post-infection, and the added amount was adopted to obtain MOIs of <NUM>, <NUM>, <NUM>, and <NUM>, respectively. Lefamulin (as acetate) was investigated in this study as well as TMC353121 for positive control.

The antiviral efficacy and cellular toxicity data are summarized in the tables below. The EC<NUM> value in the low µM range for Lefamulin was reproduced at an MOI of <NUM>. In contrast, a higher MOI, thus higher viral load with respect to the investigated cells, reduced the antiviral effect of Lefamulin. This effect is less pronounced in the highly effective control substance TMC353121.

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability following replication of the two different respiratory syncytial virus strains RSV ALONG and RSV B<NUM> in HEp2 cells.

Methodology: The assay was performed in analogy to Example <NUM> above with the difference that cells seeded with a density of <NUM> x <NUM><NUM> cells per well were incubated with the virus strains RSV ALONG or RSV B<NUM>, respectively, following a <NUM> hour cell pretreatment with the test compound at different concentrations. Virus was diluted and added in an amount yielding MOIs of <NUM> and <NUM> for RSV ALONG and RSV B<NUM>, respectively.

The antiviral efficacy and cellular toxicity data are summarized in the tables below. The control compound TMC353121 was evaluated in parallel to Lefamulin and yielded an EC<NUM> value of <NUM> against the investigated strains of RSV A and RSV B. Lefamulin yielded an EC<NUM> value of <NUM> against the RSV B<NUM>. Activity against RSV ALONG could not be determined due to the cytotoxicity to HEp2 cells with TC<NUM> values of <NUM> in the assay.

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability during replication of Measles virus strain Edmonston in HeLa cells.

Method: HeLa cells were seeded in <NUM>-well flat-bottom tissue culture plates (at a density of <NUM> x <NUM><NUM> cells per well) and allowed to adhere overnight. Thereafter, diluted test compounds (Lefamulin as acetate, Ribavirin for control) were added to the plate and incubated for <NUM> hours prior to addition of the virus. Virus was added diluted to a pre-determined titer to yield <NUM>-<NUM>% cell killing at <NUM> days post-infection (<NUM>:<NUM> dilution, MOI of <NUM>).

Cell viability determination and calculation of EC<NUM> and TC<NUM> were performed as described in Examples <NUM> and <NUM>.

The antiviral efficacy and cellular toxicity data are summarized in the Table below. Ribavirin was evaluated as control compound in parallel to Lefamulin and yielded an EC<NUM> value of <NUM>µg/mL. Surprisingly, Lefamulin yielded an even lower EC<NUM> value of <NUM> with a high calculated TI of <NUM>.

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability during replication of Dengue virus strain DENV2New Guinea in Huh7 cells.

Method: Huh7 cells were seeded in <NUM>-well flat-bottom tissue culture plates (at a density of <NUM> x <NUM><NUM> cells per well) and allowed to adhere overnight. Thereafter, diluted test compounds (Lefamulin as acetate, Ribavirin for control) were added to the plate and incubated for <NUM> hours prior to addition of the virus. The Dengue virus strain DENV2New Guinea was obtained from ATCC (VR-<NUM>) and was grown in Rhesus monkey kidney cells for the production of stock virus pools. Virus was added diluted to a pre-determined titer to yield <NUM>-<NUM>% cell killing at <NUM> days post-infection (MOI of <NUM>).

Cell viability determination as well as EC<NUM> and TC<NUM> calculations were performed as described in Examples <NUM> and <NUM>.

The antiviral efficacy and cellular toxicity data are summarized in the Table below. Ribavirin was evaluated as control compound in parallel to Lefamulin and yielded an EC<NUM> value of <NUM>µg/mL. Lefamulin yielded an EC<NUM> value of <NUM>. Ribavirin and Lefamulin both showed a certain cytotoxicity for this specific cell line at concentrations of <NUM>µg/mL and <NUM>, respectively.

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability during replication of Zika virus strain ZIK VPRVABC59 in Huh7 cells following a <NUM> hour cell pretreatment.

Method: Huh7 cells were seeded in <NUM>-well flat-bottom tissue culture plates (at a density of <NUM> x <NUM><NUM> cells per well) and allowed to adhere overnight. Thereafter, diluted test compounds (Lefamulin as acetate, Sofosbuvir for control) were added to the plate and incubated for <NUM> hours prior to addition of the virus. The Zika virus strain PRVABC59 obtained from ATCC (catalog VR-<NUM>) was obtained from ATCC (VR-<NUM>) and was grown in Rhesus monkey kidney cells for the production of stock virus pools. Virus was added diluted to a pre-determined titer to yield <NUM>-<NUM>% cell killing at <NUM> days post-infection (MOI of <NUM>).

The antiviral efficacy and cellular toxicity data are summarized in the Table below. The control compound Sofosbuvir was evaluated in parallel to Lefamulin and yielded an EC<NUM> value of <NUM>µg/mL. Lefamulin yielded an EC<NUM> value of <NUM> with a calculated therapeutic index of <NUM>.

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability during replication of human rhinovirus strain HRV16 strain <NUM> in H1-HeLa cells following a <NUM> hour cell pretreatment.

Method: H1-HeLa cells were seeded in <NUM>-well flat-bottom tissue culture plates (at a density of <NUM> x <NUM><NUM> cells per well) and allowed to adhere overnight. Thereafter, diluted test compounds (Lefamulin as acetate, Rupintrivir for control) were added to the plate and incubated for <NUM> hours prior to addition of the virus. The virus HRV16<NUM> was added diluted to a pre-determined titer to yield <NUM>-<NUM>% cell killing in the untreated virus control wells (MOI of <NUM>).

Rupintrivir, a protease inhibitor developed for treatment of rhinoviruses, was evaluated in parallel and yielded an EC<NUM> value of <NUM>. Lefamulin yielded an EC<NUM> value of <NUM> with a calculated therapeutic index of <NUM>.

Objective: The assay measured the inhibition of virus-induced cytopathic effects (CPE) and cell viability during replication of influenza virus strain A/PR/<NUM>/<NUM> in MDCK cells following a <NUM> hour cell pretreatment.

Method: MDCK cells were seeded in <NUM>-well flat-bottom tissue culture plates (at a density of <NUM> x <NUM><NUM> cells per well) and allowed to adhere overnight. Thereafter, diluted test compounds (Lefamulin as acetate, Oseltamivir for control) were added to the plate and incubated for <NUM> hours prior to addition of the virus. The influenza virus strain A/PR/<NUM>/<NUM> was added diluted to a pre-determined titer to yield <NUM>% cell killing in the untreated virus control wells (MOI of <NUM>).

Oseltamivir as established influenza drug was evaluated in parallel and yielded an EC<NUM> value of <NUM>. Lefamulin was cytotoxic to MDCK cells at concentrations greater than <NUM>. A maximum inhibition of the influenza mediated CPE by <NUM>% was measured at <NUM> Lefamulin. Therefore, and because cytotoxicity was observed at <NUM>, an EC<NUM> could not be determined for Lefamulin. However, an in vivo activity was observed in an Influenza infection mouse model (see Example <NUM> below) using a related mouse adapted Influenza A strain (Influenza A/Puerto Rico/<NUM>/<NUM> (H1N1)).

Objective: Effects of Lefamulin were investigated in an in vivo Influenza virus infection model. In the Influenza virus model, mice were challenged with an influenza A (H1N1) strain adapted to mice.

Methodology: Adult female BALB/c mice were randomly allocated to three experimental groups of <NUM> animals and allowed to acclimatize for one week. Treatments were administered subcutaneously starting at Day -<NUM>. The negative control group received a vehicle administered twice per day. Lefamulin was investigated at different dosing. In the low dose regime <NUM>/kg of Lefamulin were administered twice daily (corresponding to a dose of <NUM>/kg/day) from Day -<NUM> to Day <NUM>. In the high dose regime, Lefamulin was administered with a dose of <NUM>/mg/kg/day in three injections until day <NUM> and was altered from Day <NUM> on due to administration problems at the injection site. The following doses were <NUM>/kg administered twice daily (corresponding to <NUM>/kg/day). On Day <NUM>, all groups were challenged with influenza A/Puerto Rico/<NUM>/<NUM> (H1N1).

During the study, animals were scored daily for clinical signs of influenza virus infection to include abnormal coat condition (piloerection), abnormal posture (hunched), abnormal breathing (rapid and/or irregular breathing rate), reduced mobility, ocular discharged, eye closure and/or survival. The signs of severity of disease were added for the scoring system yielding a maximum possible score of <NUM>. When clinical signs were judged as severe, individual animals were taken out of the study prior to the scheduled end of the study.

At Day <NUM>, lung tissue was dissected, assessed for gross pathology, preserved in fixative and stored for histopathology.

Lung consolidation was scored as follows after macroscopic evaluation: ><NUM>% (across all lobes) of field occupied by intra-alveolar edema/haemorrhage; extensive vascular degeneration. Lungs removed and fixated on Day <NUM> were evaluated microscopically in the histopathology. Four main readouts were evaluated (Bronchial/Bronchiolar Degeneration/Hyperplasia, Broncho-interstitial Inflammation, Alveolar Inflammation/Degeneration, Alveolar Edema/Haemorrhage) and scored yielding a maximum total histopathology score of <NUM>, wherein a lower number indicates less signs of histopathological anomalies.

Lung samples were also processed and stored for Day <NUM> and Day <NUM> viral titre. On Day <NUM> and <NUM>, lungs were collected, homogenised and clarified to determine viral load by TCID<NUM> assay on Madin-Darby Canine Kidney (MDCK) cells.

The results of the clinical monitoring are shown in <FIG>. The positive control treatment with Oseltamivir worked as expected. A reduction was observed in clinical scores and bodyweight loss for Oseltamivir. Lefamulin did not have a significant effect on bodyweight at the investigated doses (<FIG>). At high dose, Lefamulin resulted in an increase in clinical scores and decrease in survival compared to vehicle, which might relate to the local tolerability (SC) issues of the investigated dosage, concentration and formulation (<FIG> and <FIG>). With the lower dose of Lefamulin, <NUM> % survival was achieved, whereas only <NUM> % of the vehicle group survived until day <NUM> (<FIG>).

Moreover, a significant improvement in the macroscopically evaluated lung consolidation was observed for Lefamulin at the low dose. In histopathology, a spectrum of overall individual animal scores (<NUM>-<NUM> range) were evident within the specimens examined (<FIG>). Lesions were similar to those described within the literature. Increasing severities/distribution area of alveolar pathology were correlated with increases in bronchiolar degeneration/proliferation, broncho-interstitial inflammation and alveola oedema/haemorrhage. Treatment with the high dose of Lefamulin resulted in a significant reduction in bronchial degeneration and alveolar inflammation resulting in an overall significant reduction in histopathology score in this group compared to the vehicle treated control and comparable to Oseltamivir.

Lung viral titre decreased in all groups between Day <NUM> and Day <NUM> (<FIG>). Lefamulin at both doses and Oseltamivir resulted in reduced lung viral titres when compared with the vehicle treated control.

The clinical readout and the reductive effect on the lung viral titer further supports the potential of Lefamulin in the treatment of viral diseases.

Objective: The example aims at the synthesis of Lefamulin itaconate as a potential new active pharmaceutical ingredient comprising Lefamulin in protonated form as cation and itaconate as an anion derived from the dicarboxylic itaconic acid.

To a solution of lefamulin as free base (<NUM>, <NUM> eq) in DMF (<NUM>) itaconic acid was added (<NUM> eq) and stirred at room temperature overnight. The resulting reaction mixture was added dropwise to MTBE. The obtained precipitate was filtered, washed with MTBE and dried under reduced pressure to receive Lefamulin itaconate (<NUM>) in the form of a colorless solid.

Claim 1:
A compound of formula (I)
<CHM>
wherein
n is <NUM> to <NUM>;
m is <NUM> or <NUM> with the proviso that the sulphur atom and R<NUM> are in vicinal position (if m = <NUM> then R<NUM> is in position <NUM>', and if m = <NUM> then R<NUM> is on position <NUM> ');
R is ethyl or vinyl;
R<NUM> is hydrogen or (C<NUM>-<NUM>)alkyl,
R<NUM> is hydrogen or
- (C<NUM>-<NUM>)cycloalkyl, or
- unsubstituted (C<NUM>-<NUM>)alkyl, or
- (C<NUM>-<NUM>)alkyl substituted by one or more of
- hydroxy; preferably one or two,
- methoxy,
- halogen,
- (C<NUM>-<NUM>)cycloalkyl, or
R<NUM> and R<NUM> together with the nitrogen atom to which they are attached form a <NUM> to <NUM> membered heterocyclic ring containing at least <NUM> nitrogen atom or <NUM> nitrogen and <NUM> additional heteroatom e. g. selected from N or O, or
R<NUM> is hydroxy and R<NUM> is formyl;
R<NUM> is OH, OR<NUM>, a halogen atom, or
R<NUM> is bound to <NUM>' and represents -O-(CH<NUM>)p-O- with p is <NUM> or <NUM>;
R<NUM> is unsubstituted (C<NUM>-<NUM>)alkyl or (C<NUM>-<NUM>)cycloalkyl,
or a pharmaceutically acceptable salt or solvate thereof
for the specific use in the treatment or prevention of a viral infection.