Accurate identification of fastidious Gram-negative rods: integration of both conventional phenotypic methods and 16S rRNA gene analysis.

BACKGROUND: Accurate identification of fastidious Gram-negative rods (GNR) by conventional phenotypic characteristics is a challenge for diagnostic microbiology. The aim of this study was to evaluate the use of molecular methods, e.g., 16S rRNA gene sequence analysis for identification of fastidious GNR in the clinical microbiology laboratory.
RESULTS: A total of 158 clinical isolates covering 20 genera and 50 species isolated from 1993 to 2010 were analyzed by comparing biochemical and 16S rRNA gene sequence analysis based identification. 16S rRNA gene homology analysis identified 148/158 (94%) of the isolates to species level, 9/158 (5%) to genus and 1/158 (1%) to family level. Compared to 16S rRNA gene sequencing as reference method, phenotypic identification correctly identified 64/158 (40%) isolates to species level, mainly Aggregatibacter aphrophilus, Cardiobacterium hominis, Eikenella corrodens, Pasteurella multocida, and 21/158 (13%) isolates correctly to genus level, notably Capnocytophaga sp.; 73/158 (47%) of the isolates were not identified or misidentified.
CONCLUSIONS: We herein propose an efficient strategy for accurate identification of fastidious GNR in the clinical microbiology laboratory by integrating both conventional phenotypic methods and 16S rRNA gene sequence analysis. We conclude that 16S rRNA gene sequencing is an effective means for identification of fastidious GNR, which are not readily identified by conventional phenotypic methods.

Background

Accurate identification of fastidious Gram-negative rods (GNR) is a challenge for clinical microbiology laboratories. Fastidious GNR are slow-growing organisms, which generally require supplemented media or CO2 enriched atmosphere and fail to grow on enteric media such as MacConkey agar [1]. They are isolated infrequently and consist of different taxa including Actinobacillus, Capnocytophaga, Cardiobacterium, Eikenella, Kingella, Moraxella, Neisseria, and Pasteurella. Most of them are colonizers of the human oral cavity but they have been demonstrated to cause severe systemic infections like endocarditis, septicemia and abscesses, particularly in immunocompromised patients [1,2]. Accurate identification of fastidious GNR is of concern when isolated from normally sterile body sites regarding guidance of appropriate antimicrobial therapy and patient management [1].

Identification of fastidious GNR by conventional methods is difficult and time-consuming because phenotypic characteristics such as growth factor requirements, fermentation and assimilation of carbohydrates, morphology, and staining behaviour are subject to variation and dependent on individual interpretation and expertise [1,3]. Commercially available identification systems such as VITEK 2 NH (bioMérieux, Marcy L’Etoile, France) only partially allow for accurate identification of this group of microorganisms, e.g., Eikenella corrodens, Kingella kingae and Cardiobacterium hominis[4-6]. Most studies relied only on a subset of taxa of fastidious GNR or did not include clinical isolates under routine conditions [4-6]. The application of newer identification methods like matrix-assisted laser desorption ionization-time of flight mass spectrometry (MALDI-TOF MS) shows promising results regarding the identification of HACEK group members (Haemophilus parainfluenzae, Aggregatibacter spp., Cardiobacterium spp., E. corrodens, and Kingella spp.), however, only a small set of isolates and species were investigated [7-9]. Other potentially pathogenic fastidious GNR such as Capnocytophaga spp. or Pasteurella spp., which are known agents of wound infections and septicemia after animal bites [1] frequently are not included in comparative analyses. In addition, implementation of MALDI-TOF identification also depends on the number of correctly identified reference strains in the database.

16S rRNA gene sequence analysis is generally considered as the “gold standard” for bacterial identification [3,10,11]. We analysed a substantial data set of 158 clinical fastidious GNR isolates covering various difficult-to-identify taxa, which were collected during a 17-year period. We propose a feasible strategy for accurate identification of fastidious GNR in a routine diagnostic laboratory using both conventional phenotypic and molecular methods, e.g., 16S rRNA gene analysis.

Methods

Clinical isolates

The 158 isolates of fastidious GNR included in this study derived from clinical human specimens taken as part of standard patient care and were collected from 1993 to 2010 at the Institute of Medical Microbiology, University of Zurich, Switzerland. All isolates were identified both by conventional biochemical methods and 16S rRNA gene sequence analysis. The isolates were cultured on Columbia sheep blood or chocolate agar (Becton, Dickinson & Company, Franklin Lakes, NJ (BD)) and incubated at 37°C with 5% CO2 for 24 to 48 h. The isolates were stored at −80°C as pure cultures.

Biochemical identification

The isolates were identified using in-house biochemical reactions as described for coryneform bacteria, for unusual Gram-negative aerobic bacteria and for facultative anaerobic bacteria [12,13]. In addition to the Gram stain, the following biochemical reactions were investigated: catalase, oxidase, nitrate reduction, urease, indole production, ornithine decarboxylase, hydrolysis of esculin; acid production from glucose, sucrose, maltose, mannitol and xylose was tested in semisolid cystine-trypticase agar medium (BD) supplemented with rabbit serum; tests for fermentative/nonfermentative carbohydrate metabolism were done on triple sugar iron agar. Identification by biochemical methods was scored as correct or incorrect taxonomic level compared to the 16S rRNA gene analysis as reference method. An incorrect assignment to species level was scored as incorrect species even if the genus was correct. If biochemical identification methods did not assign an isolate to at least genus level, the strain was scored as not identified.

16S rRNA gene sequence analysis

Sequencing of the partial 16S rRNA gene was performed as described previously [14]. In brief, a loopful of bacterial cells was used for extraction of DNA by lysozyme digestion and alkaline hydrolysis. Nucleic acids were purified using the QIAamp DNA blood kit (Qiagen AG, Basel, Switzerland). The 5’-part of the 16S rRNA gene (corresponding to Escherichia coli positions 10 to 806) was amplified using primers BAK11w [5´-AGTTTGATC(A/C)TGGCTCAG] and BAK2 [5´-GGACTAC(C/T/A)AGGGTATCTAAT]. Amplicons were purified and sequenced with forward primer BAK11w using an automatic DNA sequencer (ABI Prism 310 Genetic Analyzer; Applied Biosystems, Rotkreuz, Switzerland).

BLAST search of partial 16S rRNA gene sequences was performed by using Smartgene database (SmartGene™, Zug, Switzerland) on March 2013. The SmartGene database is updated with the newest 16S rRNA gene sequences from NCBI GenBank through an automated process every day. Non-validated taxa or non published sequences were not taken into consideration. The following criteria were used for 16S rRNA gene based identification [14-17]: (i) when the comparison of the sequence determined with a sequence in the database of a classified species yielded a similarity score of ≥ 99%, the isolate was assigned to that species; (ii) when the score was <99% and ≥ 95%, the isolate was assigned to the corresponding genus; (iii) when the score was < 95%, the isolate was assigned to a family. If the unknown isolate was assigned to a species and the second classified species in the scoring list showed less than 0.5% additional sequence divergence, the isolate was categorized as identified to the species level but with low demarcation. The sequence analysis was considered as the reference method but in cases with low demarcation results of supplemental conventional tests were taken into consideration for the final identification. Partial 16S rRNA gene sequences of all 158 clinical isolates were deposited in NCBI GenBank under GenBank accession numbers KC866143-KC866299 and GU797849, respectively.

VITEK 2 NH card identification

A subset of 80 of the total of 158 isolates was tested by the colorimetric VITEK 2 NH card (bioMérieux) according to the instructions of the manufacturer. The colorimetric VITEK 2 NH card contains 30 tests and the corresponding database covers 26 taxa. Identification by VITEK 2 NH was compared to the 16S rRNA gene analysis as reference method.

Results

One hundred fifty-eight clinically relevant human isolates of fastidious GNR (including rod forms of the genus Neisseria) were collected in our diagnostic laboratory during a 17-year period. Most of the 158 fastidious GNR isolates belonged to the following genera: Neisseria (n=35), Pasteurella (n=25), Moraxella (n=24), Aggregatibacter (n=20), Capnocytophaga (n=15), Eikenella (n=12), Cardiobacterium (n=6), Actinobacillus (n=3), Oligella (n=3), and Kingella (n=2) (Table 1). 16S rRNA gene analysis identified 94% of the 158 isolates to species level and 5% to genus level; one isolate could only be assigned to family level (Tables 1 and 2). Thirteen isolates were assigned to species level with low demarcation to the next species but supplemental conventional tests revealed a final identification to species level (Table 1). Conventional methods assigned 60% of the isolates to species level and 15% to genus level (Tables 1 and 2). However, only 40% were correctly assigned to species level and 13% correct to genus level considering the 16S rRNA gene sequencing as reference method. 47% of the isolates were misidentified or not identified by conventional methods; nevertheless, 18 of the 31 isolates incorrectly assigned to species level were identified to the correct genus (Table 2).

Table 1

Identification of clinical isolates (n=158) by conventional methods compared to 16S rRNA gene sequence analysis

Conventional phenotyic methods		16S rRNA gene sequence analysis			Final identification (supplemental conventional tests if required)
Identification (number of isolates)	Level of identification and correctness of result	Best reference species sequence	% difference to reference species sequence	GenBank accession numbers
Actinobacillus ureae (1)	S 1; SI 2	Actinobacillus hominis Actinobacillus suis (low demarcation)	0.0, 0.4	KC866152	A. hominis (acidification of mannitol: A. hominis (positive), A. suis (negative) [1])
Aggregatibacter actinomycetemcomitans (2)	S; SC	Aggregatibacter actinomycetemcomitans	0.0, 0.3	KC866227; KC866228	A. actinomycetemcomitans
Aggregatibacter actinomycetemcomitans (1)	S; SI	Pasteurella bettyae	0.0	KC866143	P. bettyae
Aggregatibacter aphrophilus (11)	S; SC	Aggregatibacter aphrophilus	0.0-0.8	KC866144; KC866145; KC866146; KC866147; KC866148; KC866149; KC866150; KC866229; KC866230; KC866231; KC866272	A. aphrophilus
Aggregatibacter aphrophilus (2)	S; SI	Aggregatibacter aphrophilus	3.8, 2.9	KC866151; KC866153	Aggregatibacter sp.
Aggregatibacter aphrophilus (1)	S; SI	Neisseria sicca	0.8	KC866154	N. sicca (nitrate reduction: positive (N. mucosa), negative (N. sicca, N. subflava bv. flava); sucrose acidification: positive (N. sicca, N. mucosa), negative (N. subflava bv. flava) [18])
		Neisseria subflava bv. flava	1.0
		Neisseria mucosa (low demarcation)	1.1
Aggregatibacter sp. (1)	G; GC	Aggregatibacter aphrophilus	2.3	KC866155	Aggregatibacter sp.
Bergeyella zoohelcum (1)	S; SI	Myroides odoratimimus	5.9	KC866156	Flavobacteriaceae
Bergeyella zoohelcum (1)	S; SI	Neisseria zoodegmatis	0.3	KC866157	N. zoodegmatis
Capnocytophaga canimorsus (2)	S; SC	Capnocytophaga canimorsus	0.5, 0.4	KC866158; KC866159	C. canimorsus
Capnocytophaga ochracea (1)	S; SI	Capnocytophaga gingivalis	0.6	KC866160	C. gingivalis
Capnocytophaga ochracea (1)	S; SI	Capnocytophaga ochracea	2.5	KC866161	Capnocytophaga sp.
Capnocytophaga ochracea (5)	S; SI	Capnocytophaga sputigena	0.0-0.3	KC866162; KC866163; KC866164; KC866273; KC866274	C. sputigena3
Capnocytophaga ochracea (1)	S; SI	Dysgonomonas mossii	0.6	KC866165	D. mossii
Capnocytophaga ochracea (1)	S; SI	Leptotrichia trevisanii	0.2	KC866166	L. trevisanii
Capnocytophaga sp. (2)	G; GC	Capnocytophaga sputigena	0.0, 0.6	KC866167; KC866232	C. sputigena
Cardiobacterium hominis (4)	S; SC	Cardiobacterium hominis	0.0-0.5	KC866168; KC866233; KC866275; KC866299	C. hominis
CDC Group IIe (1)	S; SI	Chryseobacterium anthropi	0.2	KC866169	C. anthropi (acidification of fructose and sucrose: positive (C. haifense), negative (C. anthropi) [19])
		Chryseobacterium haifense (low demarcation)	0.6
Comamonas sp. (1)	G; GI	Oligella urethralis	0.0	KC866170	O. urethralis
Dysgonomonas capnocytophagoides (1)	S; SC	Dysgonomonas capnocytophagoides	0.2	KC866171	D. capnocytophagoides
Eikenella corrodens (10)	S; SC	Eikenella corrodens	0.0-0.8	KC866172; KC866173; KC866174; KC866175; KC866176; KC866177; KC866178; KC866234; KC866235; KC866236	E. corrodens
Flavobacterium sp. (1)	G; GC	Flavobacterium lindanitolerans	0.4	KC866179	F. lindanitolerans
Gram-negative rods (1)	N	Actinobacillus hominis	0.3	KC866238	A. hominis
Gram-negative rods (1)	N	Actinobacillus hominis	0.0	KC866237	A. hominis (esculin hydrolysis: positive (A. suis), variable (A. hominis), negative (A. equuli); mannitol acidification: positive (A. equuli, A. hominis), negative (A. suis) [1])
		Actinobacillus suis	0.0
		Actinobacillus equuli (low demarcation)	0.5
Gram-negative rods (1)	N	Aggregatibacter actinomycetemcomitans	0.2	KC866239	A. actinomycetemcomitans
Gram-negative rods (2)	N	Aggregatibacter aphrophilus	0.3, 0.8	KC866240; KC866241	A. aphrophilus
Gram-negative rods (1)	N	Azospira oryzae	0.0	KC866276	A. oryzae
Gram-negative rods (1)	N	Brevundimonas terrae	0.6	KC866180	B. terrae
Gram-negative rods (3)	N	Capnocytophaga canimorsus	0.0-0.2	KC866277; KC866278; KC866279	C. canimorsus
Gram-negative rods (1)	N	Capnocytophaga sputigena	0.0	KC866280	C. sputigena
Gram-negative rods (2)	N	Cardiobacterium hominis	0.5, 0.6	KC866281; KC866282	C. hominis
Gram-negative rods (1)	N	Chryseobacterium haifense	0.2	KC866181	C. anthropi (acidification of fructose and sucrose: positive (C. haifense), negative (C. anthropi) [19])
		Chryseobacterium anthropi (low demarcation)	0.5
Gram-negative rods (1)	N	Kingella denitrificans	0.0	KC866182	K. denitrificans
Gram-negative rods (1)	N	Moraxella atlantae	0.2	KC866242	M. atlantae
Gram-negative rods (2)	N	Moraxella lacunata	0.0	KC866283; KC866284	M. lacunata
Gram-negative rods (1)	N	Moraxella lincolnii	0.3	KC866243	M. lincolnii
Gram-negative rods (3)	N	Moraxella nonliquefaciens	0.0-0.7	KC866285; KC866286; KC866287	M. nonliquefaciens
Gram-negative rods (2)	N	Moraxella osloensis	0.0, 0.2	KC866288; KC866289	M. osloensis
Gram-negative rods (1)	N	Neisseria bacilliformis	0.0	KC866244	N. bacilliformis
Gram-negative rods (1)	N	Neisseria zoodegmatis	2.0	KC866245	Neisseria sp.
Gram-negative rods (4)	N	Neisseria elongata	0.0-0.3	KC866246; KC866247; KC866290; KC866291	N. elongata
Gram-negative rods (1)	N	Neisseria flavescens	0.5	KC866248	N. subflava (acidification of glucose and maltose: positive (N. subflava), negative (N. flavescens) [18])
		Neisseria subflava (low demarcation)	0.7
Gram-negative rods (2)	N	Neisseria flavescens	0.3	KC866249; KC866250	N. subflava (acidification of glucose and maltose: positive (N. subflava), negative (N. flavescens) [18])
		Neisseria subflava (low demarcation)	0.4
Gram-negative rods (4)	N	Neisseria weaveri	0.0-0.3	KC866251; KC866252; KC866253; KC866254	N. weaveri
Gram-negative rods (1)	N	Pasteurella bettyae	0.0	KC866292	P. bettyae
Gram-negative rods (1)	N	Pasteurella dagmatis	0.4	KC866255	P. stomatis (urease reaction: positive (P. dagmatis), negative (P. stomatis); acidification of maltose: positive (P. dagmatis), negative (P. stomatis) [1])
		Pasteurella stomatis (low demarcation)	0.4
Kingella denitrificans (1)	S; SC	Kingella denitrificans	0.6	KC866183	K. denitrificans
Kingella denitrificans (1)	S; SI	Neisseria elongata	0.0	KC866184	N. elongata
Leptotrichia buccalis (1)	S; SI	Leptotrichia trevisanii	0.3	KC866293	L. trevisanii
Moraxella lacunata (1)	S; SC	Moraxella lacunata	0.5	KC866185	M. lacunata (gelatinase reaction: positive (M. lacunata), negative (M. nonliquefaciens) [20])
		Moraxella nonliquefaciens (low demarcation)	0.7
Moraxella osloensis (1)	S; SC	Moraxella osloensis	0.0	KC866186	M. osloensis
Moraxella osloensis (1)	S; SI	Psychrobacter faecalis	0.0	KC866187	P. pulmonis (acidification of glucose and xylose: positive (P. faecalis), negative (P. pulmonis) [20])
		Psychrobacter pulmonis (low demarcation)	0.2
Moraxella sp. (1)	G; GC	Moraxella canis	0.2	KC866188	M. canis
Neisseria sp. (1)	G; GI	Neisseria elongata	0.3	KC866256	N. elongata
Moraxella sp. (4)	G; GC	Moraxella nonliquefaciens	0.0-0.3	KC866189; KC866190; KC866257; KC866258	M. nonliquefaciens
Moraxella sp. (8)	G; GC	Moraxella osloensis	0.0-0.2	KC866191; KC866192; KC866193; KC866194; KC866259; KC866260; KC866261; KC866294	M. osloensis
Neisseria animaloris (EF4a) (1)	S; SC	Neisseria animaloris	0.0	KC866195	N. animaloris
Neisseria animaloris (EF4a) (1)	S; SI	Neisseria zoodegmatis	0.0	GU797849	N. zoodegmatis
Neisseria cinerea (2)	S; SC	Neisseria cinerea	0.0	KC866196; KC866197	N. cinerea (acidification of glucose and maltose: positive (N. meningitidis), negative (N. cinerea) [18])
		Neisseria meningitidis (low demarcation)	0.3
Neisseria elongata (1)	S; SI	Aggregatibacter aphrophilus	2.4	KC866198	Aggregatibacter sp.
Neisseria elongata (3)	S; SC	Neisseria elongata	0.0-0.3	KC866203; KC866204; KC866205	N. elongata
Neisseria elongata (2)	S; SI	Neisseria bacilliformis	0.1, 0.4	KC866201; KC866202	N. bacilliformis
Neisseria elongata (1)	S; SI	Neisseria zoodegmatis	0.6	KC866206	N. zoodegmatis
Neisseria elongata (2)	S; SI	Eikenella corrodens	0.0	KC866199; KC866200	E. corrodens
Neisseria sp. (1)	G; GC	Neisseria shayeganii	0.3	KC866207	N. shayeganii
Neisseria sp. (1)	G; GC	Neisseria elongata	0.2	KC866270	N. elongata
Neisseria sp. (1)	G; GC	Neisseria oralis	0.0	KC866208	N. oralis
Neisseria weaveri (1)	S; SC	Neisseria weaveri	0.0	KC866211	N. weaveri
Neisseria weaveri (1)	S; SC	Neisseria shayeganii	0.2	KC866210	N. shayeganii
Neisseria weaveri (1)	S; SI	Azospira oryzae	0.0	KC866209	A. oryzae
Neisseria zoodegmatis (EF4b) (3)	S; SC	Neisseria zoodegmatis	0.0-0.5	KC866212; KC866213; KC866295	N. zoodegmatis
Oligella urethralis (2)	S; SC	Oligella urethralis	0.0	KC866214; KC866215	O. urethralis
Pasteurella aerogenes (1)	S; SI	Pasteurella aerogenes	2.7	KC866226	Pasteurella sp.
Pasteurella bettyae (2)	S; SC	Pasteurella bettyae	0.0	KC866216; KC866262	P. bettyae
Pasteurella canis (1)	S; SC	Pasteurella canis	0.0	KC866217	P. canis
Pasteurella canis (1)	S; SI	Pasteurella stomatis	1.6	KC866218	Pasteurella sp.
Pasteurella dagmatis (1)	S; SC	Pasteurella dagmatis	0.2	KC866271	P. dagmatis
Pasteurella multocida (14)	S; SC	Pasteurella multocida	0.0-0.2	KC866219; KC866220; KC866221; KC866222; KC866223; KC866263; KC866264; KC866265; KC866266; KC866267; KC866268; KC866296; KC866297; KC866298	P. multocida
Pasteurella pneumotropica (1)	S; SI	Bisgaard Taxon 22	1.7	KC866224	Pasteurella sp.
Pasteurella sp. (1)	G; GI	Necropsobacter rosorum	0.0	KC866269	N. rosorum
Roseomonas sp. (1)	G; GC	Roseomonas mucosa	0.0	KC866225	R. mucosa

1Assignment to taxonomic level: S = species, G = genus, N = not identified.

2Correctness of assignment: SC = correct at species level, SI = incorrect at species level, GC = correct at genus level, GI = incorrect at genus level, N = not identified.

3 Difficult differentiation of species in question by conventional tests.

Table 2

Summary of identification of fastidious GNR isolates (n=158)

Identification procedure	% correct identification at taxonomic level		% incorrect assignment at taxonomic level or no identification
	Species	Genus	Species	Genus	No identification
16S rRNA gene sequence analysis	94% (n=148)	5% (n=9)	-	-	1% (n=1)
Conventional phenotypic methods	40% (n=64)	13% (n=21)	20% (n=31)	2% (n=3)	25% (n=39)

Conventional methods mostly misidentified Moraxella spp. and Neisseria spp.; only 2 out of 24 Moraxella spp., 3 out of 10 Neisseria elongata and 1 out of 5 Neisseria weaveri, respectively, were correctly identified to species level. In contrast, results of phenotypic identification of Aggregatibacter aphrophilus, Cardiobacterium hominis, E. corrodens, Pasteurella multocida and Capnocytophaga sp. other than Capnocytophaga canimorsus were largely congruent with 16S rRNA gene sequence analysis (Table 3). These bacteria display biochemical key reactions that differentiate them from other fastidious GNR; e.g., a positive ornithine decarboxylase reaction and missing sugar acidification in the cystine-trypticase agar medium is typical for E. corrodens; a blood culture isolate with a positive indole reaction and a negative catalase is diagnostic for C. hominis; P. multocida has a typical pattern of acidification of sugars and a positive indole reaction and together with a history of cat bite the diagnosis is feasible [1]. C. canimorsus differs from Capnocytophaga gingivalis, Capnocytophaga ochracea, Capnocytophaga sputigena by the positive catalase and oxidase – together with the typical morphology of spindle-shaped cells in the Gram stain and the anamnestic history of a dog bite, the identification is possible with conventional methods; the other Capnocytophaga spp. with a negative catalase and oxidase are difficult to differentiate by conventional methods but identification to the genus level is feasible [21].

Table 3

Taxa with mostly reliable identification of fastidious GNR by conventional phenotypic methods

Conventional phenotypic methods (number of isolates)	Final identification 1
Aggregatibacter aphrophilus (14)	A. aphrophilus (11)
	Aggregatibacter sp. (2)
	Neisseria sicca (1)
Capnocytophaga canimorsus (2)	C. canimorsus (2)
Capnocytophaga sp. (11)	C. sputigena (7)
	C. gingivalis (1)
	Capnocytophaga sp. (1)
	Dysgonomonas mossii (1)
	Leptotrichia trevisanii (1)
Cardiobacterium hominis (4)	C. hominis (4)
Eikenella corrodens (10)	E. corrodens (10)
Pasteurella multocida (14)	P. multocida (14)

1 Final identification was assigned using 16S rRNA gene identification as the reference method and if required with supplemental conventional tests.

The 80 out of 158 isolates analysed by the VITEK 2 NH card belonged to the following genera: Neisseria (n=21), Moraxella (n=13), Eikenella (n=12), Aggregatibacter (n=11), Pasteurella (n=9), Capnocytophaga (n=6), Actinobacillus (n=2), Cardiobacterium (n=2), Kingella (n=2), Dysgonomonas (n=1) and Leptotrichia (n=1) (Table 4). The VITEK 2 NH card identified 25 (31%) and 7 (9%) isolates to correct species and genus level, respectively; 4 isolates were assigned to incorrect genus and 21 isolates were not identified; 12 of the further 23 isolates incorrectly assigned to species level were identified to correct genus (Table 4). However, the VITEK 2 NH database includes taxa of only 43 of the 80 isolates studied. Regarding only taxa included in the VITEK 2 NH database, 25 (58%) and 7 (16%) out of 43 isolates were identified to correct species and genus level, respectively. The VITEK 2 NH card supports the identification of A. aphrophilus, C. hominis, E. corrodens, Capnocytophaga sp. and Kingella sp.

Table 4

Clinical isolates tested by the colorimetric VITEK 2 NH card (n=80)

VITEK 2 NH card (number of isolates)	Level of identification and correctness of result	Final identification 1
Actinobacillus ureae (1)	S 2; SI 3	A. hominis
Aggregatibacter aphrophilus (5)	S; SC	A. aphrophilus4
Aggregatibacter aphrophilus/Haemophilus parainfluenzae5 (3)	G; GC	A. aphrophilus4
Campylobacter fetus/coli (2)	G; GI	Moraxella osloensis
Capnocytophaga sp. (4)	G; GC	C. sputigena4
Capnocytophaga sp. (1)	G; GI	Dysgonomonas mossii
Capnocytophaga sp. (1)	G; GI	Leptotrichia trevisanii
Cardiobacterium hominis (2)	S; SC	C. hominis4
Eikenella corrodens (11)	S; SC	E. corrodens4
Eikenella corrodens (1)	S; SI	Neisseria elongata4
Haemophilus parainfluenzae (1)	S; SI	Actinobacillus hominis
Haemophilus parainfluenzae5 (1)	S; SI	Aggregatibacter aphrophilus4
Haemophilus parainfluenzae (1)	S; SI	Pasteurella multocida6
Kingella denitrificans (2)	S; SC	K. denitrificans4
Kingella denitrificans (2)	S; SI	Neisseria bacilliformis
Moraxella catarrhalis (1)	S; SI	M. nonliquefaciens
Moraxella catarrhalis (2)	S; SI	M. osloensis
Moraxella catarrhalis (1)	S; SI	Neisseria elongata4
Neisseria cinerea (1)	S; SC	N. cinerea4
Neisseria elongata (1)	S; SI	Capnocytophaga canimorsus4
Neisseria elongata (1)	S; SI	Capnocytophaga gingivalis4
Neisseria elongata (1)	S; SI	Eikenella corrodens4
Neisseria elongata (3)	S; SC	N. elongata4
Neisseria elongata (4)	S; SI	N. weaveri
Neisseria gonorrhoeae (1)	S; SI	Moraxella lacunata
Neisseria sicca (1)	S; SC	N. sicca4
Neisseria sicca (2)	S; SI	N. subflava
Neisseria elongata (1)	S; SI	N. zoodegmatis
Suttonella indologenes (1)	S; SI	Aggregatibacter actinomycetemcomitans4
Not identified (1)	N	Aggregatibacter aphrophilus4
Not identified (1)	N	Moraxella atlantae
Not identified (1)	N	Moraxella canis
Not identified (3)	N	Moraxella nonliquefaciens
Not identified (2)	N	Moraxella osloensis
Not identified (1)	N	Neisseria animaloris
Not identified (3)	N	Neisseria elongata4
Not identified (1)	N	Neisseria zoodegmatis
Not identified (2)	N	Pasteurella bettyae
Not identified (5)	N	Pasteurella multocida6
Not identified (1)	N	Pasteurella stomatis

1 Final identification was assigned using 16S rRNA gene identification as the reference method and if required with supplemental conventional tests.

2 Assignment to taxonomic level: S = species, G = genus, N = not identified.

3 Correctness of assignment: SC = correct at species level, SI = incorrect at species level, GC = correct at genus level, GI = incorrect at genus level, N = not identified.

4 Taxon included in the VITEK 2 NH database; Capnocytophaga spp. is included as genus.

5 Accepted as correct genus as Haemophilus aphrophilus was renamed as Aggregatibacter aphrophilus[22].

6Pasteurella multocida is included in the database of the VITEK 2 ID GNB card (bioMérieux).

Discussion

In this study, we analysed a large set of fastidious GNR clinical isolates covering diverse genera and species, which were obtained under routine conditions in a diagnostic microbiology laboratory. Molecular identification is vastly superior to conventional identification, both in number of isolates assigned to correct taxon level and in accuracy (Table 2). A minority (6%) of the 158 isolates included in the study could not be assigned to species level by 16S rRNA gene sequence analysis. In contrast, 47% of the 158 isolates were not identified or misidentified by conventional phenotypic methods (Table 2). However, the performance of supplemental phenotypic tests was helpful to support the molecular identification in cases with low demarcation of two or more species due to highly similar 16S rRNA gene sequences (Table 1).

Although the overall correct assignment to taxa by conventional phenotypic methods was rather poor, some species are easily assigned to correct species level by conventional identification procedures (Table 3). These are A. aphrophilus, C. hominis, E. corrodens, P. multocida and Capnocytophaga sp. other than C. canimorsus, which are characterised by typical biochemical key reactions that readily differentiate them from other fastidious GNR. In contrast, genera of Moraxella and Neisseria represent a challenge for the biochemical identification. Both genera often show similar biochemical reaction patterns, e.g., positive oxidase reaction or missing acid production from glucose, sucrose, maltose, mannitol, and xylose in semisolid cystine-trypticase agar medium; furthermore, the morphology in the Gram-stain does often not differentiate Moraxella and Neisseria species [13].

As alternative to conventional phenotypic methods, we analysed a subgroup of 80 isolates of fastidious GNR by the commercially available colorimetric VITEK 2 NH card (bioMérieux). Despite the limited database, this system supports the identification of fastidious GNR similar to that of conventional biochemical reactions by identifying 31% and 9% of the isolates to correct species and genus level, respectively.

Accurate identification of clinically relevant isolates of fastidious GNR is important for adequate interpretation and reporting as infectious agents and susceptibility testing [1]. However, in a routine diagnostic microbiology laboratory it is not feasible to subject all clinical isolates to molecular analyses for identification. Mahlen et al. proposed an efficient strategy by applying selective criteria such as discordant morphologic or biochemical results and knowledge of validity of phenotypic testing of isolates of Gram-negative bacilli [23]. Based on our data, we propose a cost-efficient algorithm, which is based on the knowledge of easy-to-identify organisms by conventional phenotypic methods and molecular analyses by the 16S rRNA gene for other difficult-to-differentiate species of this group. For identification of fastidious GNR conventional biochemical reactions and 16S rRNA gene sequence analysis can be implemented in a diagnostic laboratory as follows: (i) conventional biochemical identification of A. aphrophilus, C. hominis, E. corrodens, and P. multocida based on the typical reaction pattern is reliable; and (ii) any other result including Capnocytophaga sp. should be subjected to molecular methods by 16S rRNA gene analysis when accurate identification is of concern. By applying this approach to the 158 fastidious GNR analysed in our study, at least a third (32%) of the isolates would be readily identified by conventional phenotypic methods without laborious molecular analyses.

Conclusions

In time of cost-effectiveness and rapid development of newer identification methods such as MALDI-TOF MS, an efficient strategy for difficult-to-identify bacteria is mandatory as alternative method. In this study we analysed a substantial set of various clinical isolates covering 20 genera and 50 species of fastidious GNR and evaluated the reliability of both conventional phenotypic methods and 16S rRNA gene analyses for accurate identification of such microorganisms. We propose an identification algorithm for fastidious GNR for a routine diagnostic laboratory as follows: (i) conventional biochemical identification of A. aphrophilus, C. hominis, E. corrodens, and P. multocida based on the typical reaction pattern is reliable; and (ii) any other result including Capnocytophaga sp. should be subjected to molecular methods by 16S rRNA gene analysis when accurate identification is of concern.

Competing interests

The authors declare that they have no competing interests.

Authors’ contributions

MMO contributed to the acquisition of laboratory data, analysis of biochemical data and drafting the manuscript. SA contributed to the overall study design and acquisition of molecular data. GVB contributed to the overall study design and critical revision of the draft. RZ contributed to the overall study design, analysis and interpretation of biochemical data and helped to draft the manuscript. AZ contributed to the acquisition of laboratory data, molecular analyses, evaluation of the sequence data and drafting the manuscript. All authors read and approved the final manuscript.