Comparative Genomics and Phenotypic Characterization of Gluconacetobacter entanii, a Highly Acetic Acid-Tolerant Bacterium from Vinegars

The bacterial species Gluconacetobacter entanii belongs to a group of acetic acid bacteria. In 2000, it was described as a primary species of submerged spirit vinegar-producing bioreactors with a strict requirement of acetic acid, ethanol, and glucose for growth. Over the years, the type-strain of G. entanii deposited in international culture collections has lost the ability for revitalization and is thus not available any more in a culturable form. Here, we have systematically characterized phenotypic features and genomes of recently isolated G. entanii strains and compared them with characteristics of the type-strain available from published data. Using the functional annotation, genes gmhB and psp were identified as unique for G. entanii genomes among species in the clade Novacetimonas. The genome stability of G. entanii was assessed after 28 and 43 months of preculturing the strain Gluconacetobacter entanii AV429 twice a week. The strain G. entanii AV429 did not accumulate giant insertions or deletions but a few gene mutations. To unify further research into acetic acid bacteria systematics and taxonomy, we propose G. entanii AV429 as the neotype strain.


Introduction
Gluconacetobacter entanii was described as a novel bacterial species in a group of acetic acid bacteria in 2000 [1]. It was isolated from submerged high acetic acid-containing spirit vinegar bioprocesses in the Southern part of Germany. The phenotypic analysis of four strains revealed their extraordinary characteristics: the inability to grow in the absence of acetic acid, ethanol, and glucose, the requirement of total concentrations of acetic acid plus ethanol higher than 6% for growth, and the inability to over-oxidize acetic acid to CO 2 and H 2 O. The strains evolved extreme adaptation to high concentrations of acetic acid, as high as 11 vol%, being, to our knowledge, the microorganism with the highest tolerance to acetic acid ever described. According to the taxonomic requirements for novel species description, one of these strains has been described as a type-strain and deposited into international microbial culture collections [1].
Although much attention has been given to developing an improved long-term preservation protocol for G. entanii strains [2], the type-strain available from the German collection of microorganisms (DSMZ) lost its ability to be recovered on growth media from the preserved form. Today, the type-strain of G. entanii is not available in a culturable form from any of the publicly available bacterial culture collections [3,4]. This is also why this species kept the naming Gluconacetobacter entanii although the clade to which G. entanii taxonomically belongs has been in 2013 reclassified into Komagataeibacter genus [5,6] and in 2022 Bacterial strains used in this study are listed in Table 1. The strains have been revitalized from −80 • C on RAE medium (glucose 40 g/L, peptone 10 g/L, yeast extract 10 g/L, citric acid 1.37 g/L, Na 2 HPO 4 · 2 H 2 O 3.38 g/L, agar 10 g/L) containing glacial acetic acid (1 vol%) and absolute ethanol (1 vol%) with incubation at 30 • C and 92-96% relative air humidity for 3 days [2,7].
The phenotypic characterization of strains G. entanii AV429, G. entanii SI2084 and G. entanii FXV2 was principally performed as described previously [7]. Briefly, growth on various carbon sources was tested in liquid medium containing 1% of the selected carbon source, 0.5% of yeast extract, and pH adjusted to 6.8. The growth was positive if A 600 reached at least 0.3 in 7 days. An A 600 between 0.1 and 0.3 was designated as weak growth. Growth in the presence of 30% glucose (5 g/L yeast extract, 300 g/L glucose and 15 g/L agar) was tested during two-weeks incubation at 30 • C. Growth in the presence of D-glucose, D-mannitol and ethanol as a sole carbon source in the presence of ammonium sulphate as the sole nitrogen source was tested on Hoyer-Frateur and Asai culture media during ten days of incubation at 30 • C. Growth in the presence of different ethanol and acetic acid concentrations was tested in liquid RAE medium containing 1 vol% ethanol and 1.0-7.0 vol% of acetic acid or RAE medium containing 3 vol% ethanol and 1.0-7.0 vol% of acetic acid. Additionally, tests specifically described for G. entanii 4560 T by Schüller et al. [1] were performed as described above except that AE medium (2 g/L yeast extract, 3 g/L peptone and 5 g/L of the selected carbon source) with addition of 4 vol% acetic acid and 3 vol% ethanol was used as a growth medium. Gluconic acids were identified with a modified method of Gosselé et al. [11] as described by Marič et al. [12]. The presence of cellulose was checked in 5% NaOH, as described by Navarro et al. [13].
Comparison of lag phase and specific growth rates among strains AV429, SI2084 and FXV2 was estimated from growth curves in an AE medium containing 4 vol% of acetic acid and 3 vol% of ethanol generally as described previously [14]. More specifically, a 250-mL baffled flask containing 50 mL AE broth with acetic acid and ethanol was inoculated with 500 µL of bacterial culture with a density of 0.4 at A 600 and incubated at 30 • C and 180 rpm. The bacterial growth was monitored by the optical density at A 600 . The exponential growth phase was identified in log(A 600 ) vs. time plot. The specific growth rates (µ) were calculated by linear regression of ln(A 600 ) vs. time, with growth rate as the regression coefficient. All strains grew in this medium planktonically.
For genome stability experiments, strain G. entanii AV429 was precultured on an RAE medium containing 1 vol% of ethanol and 1 vol% of acetic acid twice a week for 43 months. For further analysis, DNA extracted from the biomass harvested after 28 months (strain designation G. entanii AV429-2020) and 43 months (G. entanii AV429-2022) was used.

Genome Sequences, Assembly and Annotation
Whole genome sequencing of strains G. entanii KS542, G. entanii KS544, G. entanii KS545, G. entanii AV429-2020 and G. entanii AV429-2022 was performed at the Department for Microbiology, Faculty of Medicine, University of Maribor. The DNA of the strains was isolated from the exponential growth phase using the GeneJET Genomic DNA Purification Kit (Thermo Scientific, Waltham, MA, USA) and subjected to genome sequence analysis. The paired-end libraries were prepared with the Nextera XT DNA Library Preparation Kit (Illumina, San Diego, CA, USA) following the manufacturer's protocol. The sequencing was performed on Illumina NextSeq2000 (Illumina, San Diego, CA, USA). Fastq reads were quality-checked and trimmed with Trimmomatic [17], followed by the genome assembly using SPAdes version number 3.13.1 (https://cab.spbu.ru/software/spades/) [18] with default parameters and the option "careful"; the option tries to reduce the number of mismatches and short indels. The genome sequences were deposited into the GenBank database under the accession numbers presented in Table 2. The accession numbers for strains G. entanii KS542, G. entanii KS544, G. entanii KS545, G. entanii AV429-2020, and G. entanii AV429-2022 are JANGSU000000000, JANGST000000000, JANGSS000000000, JANGSR000000000, JANGSQ000000000, respectively. Assembly was performed at the NCBI using the Prokaryotic Genome Annotation Pipeline (PGAP).

Phylogenomic Studies
The overall genome similarities among G. entanii strains were measured by orthologous average nucleotide identity algorithm (OrthoANI) using EZBioCloud [19]. For each sequenced genome, contigs longer than 500 bp were extracted and used for OrthoANI calculation. Genome distances between G. entanii strains were calculated by the Genometo-Genome Distance Calculator 2.1. The method reliably mimics conventional DNA-DNA hybridization [20].
A phylogenetic tree was constructed using concatenated core genes. The procedure started with local annotation of genome sequences by Prokka [21], followed by alignment at the minimum BlastP [22] identity of 90% by Roary [23]. From the concatenated core genes the phylogeny was inferred with the maximum likelihood algorithm included in PhyML [24] using the GTR nucleotide substitution model.

Comparative Genomic Analysis
A primary search for insertion sequences (IS) in the genomes of different G. entanii strains was performed by the program ISfinder [25]. The following criteria were further used to identify and confirm the presence and the number of homologous IS-elements by using program Geneious Prime [26]: E value below 10 −50 , query coverage over 40%, and pairwise nucleotide identity over 60%. In the strain G. entanii AV429, each of the identified IS-elements was further followed through sequence analysis of the precultured strain.
The presence of putative plasmids in G. entanii genome sequences was assessed from the presence of Rep proteins in their genome sequences. First, a database of Rep proteins originating from Acetobacter, Komagataeibacter, and Novacetimonas plasmid sequences available in NCBI was constructed. To identify identical proteins, the Rep proteins were aligned by ClustalX. Proteins differentiating in at least one amino acid were used as queries for searching homologues in the G. entanii genomes applying the same criteria as for the IS elements, except that the minimal requirement for amino acid identity was set at 40%.
Distribution of prophages in G. entanii genomes was evaluated by the Phaster webbased tool [27]. The identified prophages were categorized as intact, questionable, and incomplete depending on the representation of phage proteins in the bacterial genome. The intact prophages were further annotated using RAST server [28].
To identify specific genes in G. entanii strains, the functional annotation of the genomes was conducted by GhostKOALA [29]. The genomes of the strains were then categorized based on the presence/absence of KOs (abbreviation for KEGG Orthology), which were searched using a python script [4]. In this way, the KOs which exist in all G. entanii strains and are absent from all Novacetimonas strains of which genomes are available at NCBI were identified. In a second approach, marker genes for G. entanii were selected based on KO existence in 75% of the G. entanii strains and the absence of KO in more than 25% of Novacetimonas strains.
Principal Component Analysis (PCA) was applied to the functional annotation data. More precisely, BlastKOALA was used to annotate the CDSs of each strain with KO identifiers. Each genome and its set of annotated KOs were then used in a PCA analysis using the SIMCA 17. 0. 1 (Goettingen, Germany). This way, the strains based on the KO presence/absence and KO copy number were grouped. Strains with similar functional annotations tended to group closer and vice versa. The number of principal components used for the modeling was optimized by leave-one-observation-out cross-validation.

Phylogenomic Studies
The genomes of G. entanii strains LTH 4560 T , AV429, FXV2, SI2084, KS542, KS544, and KS545 were subjected to phylogenomic analysis. The orthoANI values among these strains ranged from 98.31% to 100% (Table S1). These results confirm that all these strains belong to the species Gluconacetobacter entanii since all values are above the 95-96% cut-off value for species demarcation [30]. Besides, the four strains SI2084, KS542, KS544, and KS545 exhibit very high similarities, from 99.8% to 100%. These strains were isolated from the same bioreactor for apple cider vinegar production [16], suggesting their clonal relatedness. The strains LTH 4560 T , AV429, and FXV2 have different geographical origins and isolation sources ( Table 1). The OrthoANI values among these strains and one of the strain mentioned above, SI2084, ranged from 98.33% to 98.60%, confirming their genetic differences.
The in silico DNA-DNA hybridization among genomes of G. entanii strains (Table S2) coincides with the findings of the orthoANI analyses. All values are above 70%, being a threshold for strain allocation into the same species [20]. Besides, high genome to genome A phylogenetic tree based on 238 core genes groups all G. entanii strains into a single subclade of the clade encompassing the genus Novacetimomas. Besides G. entanii, the clade includes species N. hansenii, N. cocois, N. pomaceti, and N. maltaceti (Figure 1). and isolation sources ( Table 1). The OrthoANI values among these strains and one of the mentioned above, SI2084, ranged from 98.33% to 98.60%, confirming their genetic diffe The in silico DNA-DNA hybridization among genomes of G. entanii strains (Ta coincides with the findings of the orthoANI analyses. All values are above 70%, b threshold for strain allocation into the same species [20]. Besides, high genome to g similarities among the strains SI2084, KS542, KS544, and KS545 are confirming th strains are of the same clonal group. A phylogenetic tree based on 238 core genes groups all G. entanii strains into a subclade of the clade encompassing the genus Novacetimomas. Besides G. entanii, the includes species N. hansenii, N. cocois, N. pomaceti, and N. maltaceti (Figure 1).

Morphological, Biochemical and Physiological Characterization of G. entanii
All strains were Gram-staining negative rods, in length 1.79-3.88 μm and wid 1.11 μm as determined by microscopy with 1000 magnification. They were all ca positive and oxidase-negative. Further phenotypic analysis was performed wi strains AV429, SI2084, and FXV2, which were, as described above, identif distinctively genomically different.
To determine if the strains are similar to the type strain G. entanii LTH 456 phenotypic characterization was performed in AE medium containing 4% acetic ac 3% ethanol. As presented in Table 3, only two phenotypic characteristics, typical type strain, matched all strains of G. entanii studied here. Additionally, the phen characteristics usually analyzed for other acetic acid bacteria [7] have been analyz the G. entanii strains. In this case, the characteristics also differ among strains (Tabl

Morphological, Biochemical and Physiological Characterization of G. entanii
All strains were Gram-staining negative rods, in length 1.79-3.88 µm and width 0.7-1.11 µm as determined by microscopy with 1000 magnification. They were all catalasepositive and oxidase-negative. Further phenotypic analysis was performed with the strains AV429, SI2084, and FXV2, which were, as described above, identified as distinctively genomically different.
To determine if the strains are similar to the type strain G. entanii LTH 4560 T , the phenotypic characterization was performed in AE medium containing 4% acetic acid and 3% ethanol. As presented in Table 3, only two phenotypic characteristics, typical for the type strain, matched all strains of G. entanii studied here. Additionally, the phenotypic characteristics usually analyzed for other acetic acid bacteria [7] have been analyzed for the G. entanii strains. In this case, the characteristics also differ among strains (Table 4).
A comparison of the growth curves ( Figure 2) among G. entanii strains (AV429, SI2084, FXV2) in liquid medium AE containing 4% acetic acid and 3% ethanol revealed differences among the strains in the length of the lag phase but similar specific growth rates. Among the three G. entanii strains, the strain SI2084 has the shortest adaptation time to 4% of acetic acid.

2023, 11, x FOR PEER REVIEW
A comparison of the growth curves ( Figure 2) among G. entanii strains FXV2) in liquid medium AE containing 4% acetic acid and 3% ethanol differences among the strains in the length of the lag phase but similar rates. Among the three G. entanii strains, the strain SI2084 has the short time to 4% of acetic acid. The strains AV429 and FXV2 form a very thick cellulose pellicle ( medium containing 1% acetic acid and 1% ethanol after 14 days of cu shown). A similar pellicle was detected with the strain AV429 also in m 2.5% acetic acid and 1% ethanol after 12 days. The pellicle was co combined with filamentous structures. It looks smooth from the top an The strains AV429 and FXV2 form a very thick cellulose pellicle (~1 cm) in an RAE medium containing 1% acetic acid and 1% ethanol after 14 days of cultivation (data not shown). A similar pellicle was detected with the strain AV429 also in medium containing 2.5% acetic acid and 1% ethanol after 12 days. The pellicle was composed of layers combined with filamentous structures. It looks smooth from the top and structured from the bottom (Figure 3). The formation of such a thick cellulose pellicle in a few days is an interesting bacterial characteristic for biomaterial production with potential applications in medicine, cosmetics, the food industry, and electronics. shown). A similar pellicle was detected with the strain AV429 also in medium containing 2.5% acetic acid and 1% ethanol after 12 days. The pellicle was composed of layers combined with filamentous structures. It looks smooth from the top and structured from the bottom (Figure 3). The formation of such a thick cellulose pellicle in a few days is an interesting bacterial characteristic for biomaterial production with potential applications in medicine, cosmetics, the food industry, and electronics.

Basic Genome Characteristics
The basic characteristics of the four G. entanii genomes are shown in Table 2. The features are very similar among the strains. In comparison to other acetic acid bacteria [7,31], the genome size of G. entanii strains (approx. 3.65 Mbp) is somewhere in the middle,

Basic Genome Characteristics
The basic characteristics of the four G. entanii genomes are shown in Table 2. The features are very similar among the strains. In comparison to other acetic acid bacteria [7,31], the genome size of G. entanii strains (approx. 3.65 Mbp) is somewhere in the middle, as the smallest genome K. kakiaceti has size of 3.13 Mbp and the biggest K. europaeus of size 4.22 Mbp. The G + C content is 62.5% or 62.6%, which is in the range of other acetic acid bacteria [7]. However, this number is rather high compared to other bacteria, given the relatively small genome size. For example, E. coli, which also represents a bacterium that adapts to a free-living environment, has a G + C content of only approximately 50%. However, its genome size is bigger, 4.6-5.5 Mbp [32]. This suggests that in the genomes of G. entanii and other acetic acid bacteria, a higher number of horizontally transmitted genes, such as transposases, drug-resistance genes, and others, such as prophages and genes encoding transporters, have accumulated through their evolution [33]. The increased G + C content also follows previous findings that aerobic prokaryotes generally possess a higher G + C% compared to anaerobic prokaryotes [34]. The proportion of pseudogenes varies between 2.9% and 4.7%, which is similar to E. coli and other non-pathogenic, nonintracellular, and non-symbiotic bacteria [35].

Mobilome Analysis
Plasmids represent one of the mobile elements in bacteria and the primary vector of horizontal gene transfer. They are essential for conferring diversity and evolution of bacteria. In the NCBI database there is presently only one strain of the genus Novacetimons (Novacetimonas hansenii C110) available with plasmid sequences. The plasmid profile of G. entanii LTH4560 T presented in the original paper also indicates a presence of more plasmids. To gain information into the plasmid repertoire of G. entanii strains, we built a database of Rep proteins from plasmids available in the NCBI database for species of Acetobacter, Gluconacetobacter, and Novacetimonas. Using rigorous criteria, we searched the homologues in the genomes of G. entanii. We identified the highest number of Rep proteins differentiating in at least one amino acid in G. entanii LTH4560 T , followed by G. entanii SI2084, G. entanii AV429, and G. entanii FXV2 (Table S3). Although this data cannot directly correlate with the number of plasmids, since the same plasmid may possess more Rep proteins and the plasmid might be part of the chromosome, the results confirm genomic diversity among the strains. In addition, the results indicate a relatively high number of putative plasmids in these strains. Further genome sequencing is necessary to obtain complete closed genomes, thus enabling precise analysis on the number of conjugative, mobilizable, and non-mobilizable plasmids in G. entanii strains.
Insertion sequences (IS) are another widespread mobile element in bacteria. Their classification is based on the transposases that catalyze their movement through the genome. The genomes can have a significant number of truncated and partial IS-elements without transposases. Here we have searched only the entire IS-elements. We identified the highest number of the whole IS-elements in type strain G. entanii LTH4560 T , followed by G. entanii SI2084, G. entanii AV429, and G. entanii FXV2 ( Table 5). None of these IS elements were present in all G. entanii strains. In G. entanii LTH4560 T , two IS-elements, ISGxy1 and IS1031A, were identified in four copies. The IS1031A has been previously associated with the inactivation of cellulose production [36].
Prophages are another type of mobile bacterial element. They promote gene transfer in and among bacterial populations [37,38]. A recent study revealed phage-like particles in 15 of 177 acetic acid bacterial strains. They all show morphology similar to Myoviridaetype phage [39]. Here we have identified one or two types of complete prophages and up to five incomplete prophages in G. entanii strains ( Table 6). Further investigation of these genetic elements revealed that the sequences contain the putative gene for phage terminase large subunit; one is similar to a homologue of Komagataeibacter phage phiKM1 (BCZ75968.1) and the other to a homologue of phage of Myoviridae sp. (DAQ38419.1) identified in the human metagenome (Table 7). One type of prophage identified here shows very high overall nt-identity to Komagataeibacter phage phiKM1, the phage of the family Myoviridiae (Table 7). Table 5. Distribution of IS-elements among Gluconacetobacter entanii strains. Table 6. Number of prophages identified in Gluconacetobacter entanii strains.

A Comparative Genomic Functional Analysis
The functional annotation of nine G. entanii strains and 15 strains of Novacetimonas species, including all presently recognized type strains, resulted in the prediction of a total number of 1741 KOs, of which three were unique for G. entanii (Table 8), and six were present in 75% of G. entanii and less than 25% of Novacetimonas strains (Table 9). Of the three unique genes, the gmhB is coding for a putative D-glycero-D-manno-heptose 1,7bisphosphate phosphatase. The gene and its product were characterized in some bacteria, from which we know it to be involved in the biosynthesis of the ADP-L-glycerol-ß-D-mannoheptose precursor of the inner core lipopolysaccharide (LPS) [40][41][42][43]. According to this data, this component is a unique component of the G. entanii LPS in the clade encompassing Novacetimonas species. This component may be involved in high acetic acid resistance. The second unique gene psp of G. entanii codes for a putative phosphoserine phosphatase with the highest query cover (83%) and amino-acid-identity (29.8%) to the phosphoserine phosphatase (PSP) of Hydrogenobacter thermophilus, representing a novel type of PSP [44]. The enzyme is supposed to catalyze the dephosphorylation of phosphoserine to serine and inorganic phosphate as part of the serine pathway in microorganisms. However, this particular type of PSP had been annotated as cofactor-dependent, possesses neither mutase activity nor the residues important for the activity, and has been since 2012 consequently defined as a novel-type PSP [44]. The third gene identified in this clade and being specific for G. entanii has no significant identity to any characterized protein.  Table 9. KOs that exist in 75% of the Gluconacetobacter entanii strains (n = 9) and do not exist in more than 25% of Novacetimonas strains (n = 15).

K03273
GmhB; D-glycero-D- Interestingly, the G. entanii genomes have, on average, an additional four copies of parA, three copies of parB, and three copies of hupB, when compared to Novacetimonas spp. (Tables S4 and S5). The primary role of ParA and ParB in bacteria is the segregation of newly replicated DNA [45,46]. For the HupB, it has been suggested to be involved in coordinating replication with DNA segregation [47]. All these findings support our above mentioned observation that G. entanii strains may possess more plasmids. Interestingly, significantly overrepresented in G. entanii strains with three additional copies on average is also gabD, putatively coding for succinate-semialdehyde dehydrogenase, which may be involved in glutaric acid production from lysin [48].
The PCA model with two principal components explains 54% of the variance present in the functional annotation data. Figure 4 shows the score plot for the two components of the PCA model, showing three clusters of observations, which corroborates the results obtained in the phylogenomic and core gene analysis, grouping together closely related strains. The obtained results indicate that the functional genomic properties of the strains are intimately related to their phylogeny.

Genome Stability of G. entanii AV429
Several papers on acetic acid bacteria have reported on the genetic instability of acetic acid bacteria, mainly due to the presence of transposons and plasmids [49,50]. To check the genome stability of G. entanii, the strain AV429 was systematically precultured for several months on an agar medium containing 1% ethanol and 1% acetic acid. After 43 months of preculturing, no giant insertions, or deletions happened ( Figure S1), which is probably a result of keeping the strain under non-harsh conditions, but rather in an environment with high glucose content and moderate concentrations of ethanol and acetic acid; this resembles conditions during vinegar production, from where most of the presently identified G. entanii strains originate. A very few gene mutations have been identified, such as in genes coding efflux pump membrane protein, dehydrogenases, transposases, and the others, whose potential effects are yet to be identified.

Conclusions
Here, we have explored the characteristics of novel G. entanii strains and compared them with those described for the type-strain. The three novel G. entanii strains of different clonal origins have highly similar genome characteristics. However, their phenotypic traits, which are usually analyzed for taxonomic purposes in the group of acetic acid bacteria, differ substantially. Recently, novel recommendations have been introduced into bacterial taxonomy, giving solid weight to genome analysis [51]. The G. entanii genomes presented here undoubtedly show high similarity to the genome sequence of the typestrain, which is unavailable in a culturable form from any of the publicly available culture collections. Two species-specific marker genes, gmhB and psp, were identified in all presently known G. entanii genomes. In the era of affordable genome sequencing, these two genes allow us quick differentiation of this species from other validly published species in the clade Novacetimonas.
Since we need a culturable strain to unify the taxonomic research into G. entanii, we propose the Gluconacetobacter entanii AV429 (ZIM B1055, LMG 31305, CCM 8957) as a

Genome Stability of G. entanii AV429
Several papers on acetic acid bacteria have reported on the genetic instability of acetic acid bacteria, mainly due to the presence of transposons and plasmids [49,50]. To check the genome stability of G. entanii, the strain AV429 was systematically precultured for several months on an agar medium containing 1% ethanol and 1% acetic acid. After 43 months of preculturing, no giant insertions, or deletions happened ( Figure S1), which is probably a result of keeping the strain under non-harsh conditions, but rather in an environment with high glucose content and moderate concentrations of ethanol and acetic acid; this resembles conditions during vinegar production, from where most of the presently identified G. entanii strains originate. A very few gene mutations have been identified, such as in genes coding efflux pump membrane protein, dehydrogenases, transposases, and the others, whose potential effects are yet to be identified.

Conclusions
Here, we have explored the characteristics of novel G. entanii strains and compared them with those described for the type-strain. The three novel G. entanii strains of different clonal origins have highly similar genome characteristics. However, their phenotypic traits, which are usually analyzed for taxonomic purposes in the group of acetic acid bacteria, differ substantially. Recently, novel recommendations have been introduced into bacterial taxonomy, giving solid weight to genome analysis [51]. The G. entanii genomes presented here undoubtedly show high similarity to the genome sequence of the type-strain, which is unavailable in a culturable form from any of the publicly available culture collections. Two species-specific marker genes, gmhB and psp, were identified in all presently known G. entanii genomes. In the era of affordable genome sequencing, these two genes allow us quick differentiation of this species from other validly published species in the clade Novacetimonas.
Since we need a culturable strain to unify the taxonomic research into G. entanii, we propose the Gluconacetobacter entanii AV429 (ZIM B1055, LMG 31305, CCM 8957) as a neotype strain for the species Gluconacetobacter entanii. This strain was genetically stable during preculturing for at least 43 months. The recognition of our proposal will enable the