Complete genome sequence of Haliscomenobacter hydrossis type strain (OT)

Haliscomenobacter hydrossis van Veen et al. 1973 is the type species of the genus Haliscomenobacter, which belongs to order "Sphingobacteriales". The species is of interest because of its isolated phylogenetic location in the tree of life, especially the so far genomically uncharted part of it, and because the organism grows in a thin, hardly visible hyaline sheath. Members of the species were isolated from fresh water of lakes and from ditch water. The genome of H. hydrossis is the first completed genome sequence reported from a member of the family "Saprospiraceae". The 8,771,651 bp long genome with its three plasmids of 92 kbp, 144 kbp and 164 kbp length contains 6,848 protein-coding and 60 RNA genes, and is a part of the Genomic Encyclopedia of Bacteria and Archaea project.


Introduction
Strain O T (= DSM 1100 = ATCC 27775) is the type strain of Haliscomenobacter hydrossis which is the type and only species within the genus Haliscomenobacter [1,2]. The generic name derives from the Greek word haliskomai, to be imprisoned, and the Neo-Latin bacter, a rod, meaning the imprisoned rod. The species epithet is derived from the Greek word hudôr, water, and Oss, a town in the Netherlands, hydrossis, from water of Oss. The imprisoned rod from the water of Oss. Five morphologically and physiologically congruent strains belonging to the species, including the type strain O T , were isolated from activated sludge samples in the early 1970s [1]. H. hydrossis was sporadically ob-served in aeration tanks of sewage treatment plants in Germany [3] and in paper industry wastewater treatment plants in France [4]. As a recent biotechnological application, biomass bulking caused by H. hydrossis was controlled by lytic bacteriophages [5]. An improved high quality draft sequence of Saprospira grandis strain Sa g1 (=HR1, DSM 2844, GOLD ID Gi033955) is the only other genomic information currently available from the family "Saprospiraceae". Here we present a summary classification and a set of features for H. hydrossis O T , together with the description of the complete genomic sequencing and annotation.

Classification and features
The single genomic 16S rRNA sequence of H. hydrossis O T was compared using NCBI BLAST [6] under default settings (e.g., considering only the highscoring segment pairs (HSPs) from the best 250 hits) with the most recent release of the Greengenes database [7] and the relative frequencies of taxa and keywords (reduced to their stem [8]) were determined, weighted by BLAST scores. The most frequently occurring genera were Haliscomenobacter (83.9%) and Lewinella (16.1%) (3 hits in total). Regarding the two hits to sequences from members of the species, the average identity within HSPs was 99.2%, whereas the average coverage by HSPs was 98.1%. Among all other species, the one yielding the highest score was Lewinella antarctica (EF554367), which corresponded to an identity of 89.1% and an HSP coverage of 66.6%. (Note that the Greengenes database uses the INSDC (= EMBL/NCBI/DDBJ) annotation, which is not an authoritative source for nomenclature or classification). The highest-scoring environmental sequence was AJ786323 ('Lake Wolfgangsee freshwater enrichment clone MS-Wolf2-H'), which showed an identity of 98.8% and an HSP coverage of 97.9%. The most frequently occurring keywords within the labels of environmental samples which yielded hits were 'lake' (10.6%), 'tin' (5.3%), 'microbi' (3.4%), 'freshwat' (3.2%) and 'mat' (3.2%) (247 hits in total). The most frequently occurring keywords within the labels of environmental samples which yielded hits of a higher score than the highest scoring species were 'lake' (11.1%), 'tin' (5.6%), 'microbi' (3.5%), 'freshwat' (3.4%) and 'mat' (3.3%) (225 hits in total). These keywords reflect the ecological properties reported for strain O T in the original description [1]. Figure 1 shows the phylogenetic neighborhood of H. hydrossis in a 16S rRNA based tree. The sequences of the two 16S rRNA gene copies in the genome differ from each other by two nucleotides and do not differ from the previously published 16S rRNA sequence AJ784892, which contains two ambiguous base calls. Phylogenetic tree highlighting the position of H. hydrossis relative to the type strains of the other species within the family "Saprospiraceae". The tree was inferred from 1,399 aligned characters [9,10] of the 16S rRNA gene sequence under the maximum likelihood (ML) criterion [11]. Rooting was done initially using the midpoint method [12] and then checked for its agreement with the current classification ( Table 1). The branches are scaled in terms of the expected number of substitutions per site. Numbers adjacent to the branches are support values from 150 maximum likelihood bootstrap replicates [13] (left) and from 1,000 maximum parsimony bootstrap replicates [14] (right) if larger than 60%. Lineages with type strain genome sequencing projects registered in GOLD [15] are labeled with one asterisk, those also listed as 'Complete and Published' with two asterisks. Standards in Genomic Sciences The cells of H. hydrossis are rod-shaped, 0.35 -0.45 µm wide and 3 -5 µl long, mostly occurring in chains and nearly always enclosed by a narrow hyaline sheath ( Figure 2) [1]. The sheath is sometimes disrupted by branching cells [1]. Flagella were never visible in EM images nor was motility ever observed [1]. Growing bacteria excrete so far unidentified polysaccharides [1]. Strain O T grows strictly aerobically and produces intracellular carotenoid pigments [1]. Optimal growth temperature was 26°C, with a span of 8-30°C [1]. Optimal pH for growth was 7.5 [1]. Organic acids, peptides, proteins, mono-and polysaccharides were reported as carbon and energy sources [1]. Starch and gelatine were decomposed by all strains of the species [1], sorbitol, glycerol, lactate, acetate, succinate and β-hydroxybutyrate were not utilized [1]. The authors of the original description of the strain suggested that O T accumulates polysaccharides either intra-or extracellularily [1].

Genome sequencing and annotation Genome project history
This organism was selected for sequencing on the basis of its phylogenetic position [25], and is part of the Genomic Encyclopedia of Bacteria and Archaea project [26]. The genome project is deposited in the Genome On Line Database [15] and the complete genome sequence is deposited in Gen-Bank. Sequencing, finishing and annotation were performed by the DOE Joint Genome Institute (JGI). A summary of the project information is shown in Table 2.  Evidence codes -IDA: Inferred from Direct Assay (first time in publication); TAS: Traceable Author Statement (i.e., a direct report exists in the literature); NAS: Non-traceable Author Statement (i.e., not directly observed for the living, isolated sample, but based on a generally accepted property for the species, or anecdotal evidence). These evidence codes are from of the Gene Ontology project [23]. If the evidence code is IDA, the property was directly observed by one of the authors or an expert mentioned in the acknowledgements.

Growth conditions and DNA isolation
H. hydrossis O T , DSM 1100, was grown in DSMZ medium 134 (Haliscomenobacter Medium) [27] at 26°C. DNA was isolated from 0.5-1 g of cell paste using MasterPure Gram-positive DNA purification kit (Epicentre MGP04100) following the standard protocol as recommended by the manufacturer, with modification st/DL for cell lysis as described in Wu et al. [26]. DNA is available through the DNA Bank Network [28].

Genome sequencing and assembly
The genome was sequenced using a combination of Illumina and 454 sequencing platforms. All general aspects of library construction and sequencing can be found at the JGI website [29]. Pyrosequencing reads were assembled using the Newbler assembler (Roche). The initial Newbler assembly consisting of 153 contigs in three scaffolds was converted into a phrap [30] assembly by making fake reads from the consensus, to collect the read pairs in the 454 paired end library. subcloning. Gaps between contigs were closed by editing in Consed, by PCR and by Bubble PCR primer walks (J.-F. Chang, unpublished). A total of 589 additional reactions were necessary to close gaps and to raise the quality of the finished sequence. Illumina reads were also used to correct potential base errors and increase consensus quality using a software Polisher developed at JGI [33]. The error rate of the completed genome sequence is less than 1 in 100,000. Together, the combination of the Illumina and 454 sequencing platforms provided 203.8 × coverage of the genome. The final assembly contained 1,005,536 pyrosequence and 35,370,321 Illumina reads.

Genome annotation
Genes were identified using Prodigal [34] as part of the Oak Ridge National Laboratory genome annotation pipeline, followed by a round of manual curation using the JGI GenePRIMP pipeline [35]. The predicted CDSs were translated and used to search the National Center for Biotechnology Information (NCBI) non-redundant database, Uni-Prot, TIGR-Fam, Pfam, PRIAM, KEGG, COG, and In-terPro databases. Additional gene prediction analysis and functional annotation was performed within the Integrated Microbial Genomes -Expert Review (IMG-ER) platform [36].

Genome properties
The genome consists of an 8,371,686 bp long circular chromosome and three plasmids of 164,019 bp, 143,757 bp and 92,189 bp length, respectively, with a G+C content of 47.1% (Table 3 and Figure  3). Of the 6,918 genes predicted, 6,858 were protein-coding genes, and 60 RNAs; 106 pseudogenes were also identified. The majority of the proteincoding genes (58.6%) were assigned with a putative function while the remaining ones were annotated as hypothetical proteins. The distribution of genes into COGs functional categories is presented in Table 4.