Epidemiological association of Campylobacter jejuni groups with pathogenicity-associated genetic markers.

BACKGROUND: Campylobacter jejuni, the most leading cause for bacterial gastroenteritis worldwide, shows a high genetic diversity among its isolates. Recently, we demonstrated the existence of six C. jejuni-groups by combining MLST with six genetic markers. These groups were further characterized by the detection of cj1321-cj1326, fucP, cj0178, cj0755/cfrA, ceuE, pldA, cstII, and cstIII in order (I.) to show further associations between these different genetic markers and MLST CCs. Moreover, different studies were able to associate several of these markers: a sialylated lipoologosaccharide (cstII/III(+)), the gamma-glytamyl-transpeptidase (ggt(+)), and the absence of a certain allele of the enterochelin-uptake-binding-protein (ceuE(11168)(-)) with severe campylobacteriosis, bloody diarrhea and unpleasant outcome. Additionally more than half of human Campylobacter-isolates were assigned to a non-livestock clade associated with the absence of cj1321-cj1326. These isolates were considered as mere colonizers.From the combination of marker genes, the ratio of human isolates in a specific group, and clinical data (II.) it should be demonstrated to which of the previous defined groups these Campylobacter-subpopulations, associated with higher virulence, correspond.
RESULTS: Besides the marker gene pldA, all new estimated genetic markers show significant differences in their distribution among the various MLST-based groups. Especially the genes for cj1321-cj1326, fucP, cj0178, cj0755/cfrA are widely associated with each other and split the study population into two major and seven intermediate groups substantiating the previous group-definition, whereas cstII and cstIII indicate at least three groups following an independent distribution pattern.
CONCLUSIONS: Based on these data a group of C. jejuni-isolates characterized by the presence of ansB, dmsA, ggt, and the absence of cj1365c, cj1585c, cj1321-cj1326, fucP, cj0178, cj0755/cfrA, and cstII/III was associated with a higher prevalence in human campylobacteriosis, bloody diarrhea as well as hospitalization and bears obviously a higher virulence for humans. In contrast to that better livestock-adapted groups characterized by the ability to utilize L-fucose and the presence of all of the five identified putative C. jejuni iron-uptake systems as well as cj1321-cj1326, cj1365c, cj1585c, and cstII and/or cstIII (sialylated lipoologosaccharide) is more prevalent in animal hosts and was secondary associated with less severe campylobacteriosis.

Background

The Gram-negative Epsilonproteobacterium Campylobacter jejuni, which is due to recent epidemiological data the most leading cause for bacterial gastroenteritis and Guillain-Barré-syndrome (GBS) worldwide, shows a high genetic diversity among its isolates [1]. As consequence of this genetic and phenotypic diversity several C. jejuni subpopulations could be identified on the basis of the presence of non-ubiquitous genes [2]. In a previous study we could identify six C. jejuni groups combining multilocus sequence typing (MLST) with six genetic markers: ansB, dmsA,ggt, cj1585c, cj1365c and dimeric tlp7 (Tlp7m + Tlp7c) [2]. Here we could in particular demonstrate that the genes ansB, dmsA,ggt occur together in a specific cj1585c- and cj1365c–negative isolate group [2].

Several studies were able to correlate further genetic markers with clinical parameters. Thus, the question was addressed how a sialylated lipoologosaccharide (LOS) affects the severity of the Campylobacter-trigged diarrhea [3-5]. It was demonstrated that a sialylated LOS of the Campylobacter cell wall is associated with an increased occurrence of bloody diarrhea and a longer duration of symptoms [3-5].

Champion and coworkers made a further interesting finding. They demonstrated that 55.7% of C. jejuni isolates from human faeces belong to a non-livestock clade that misses the flagellin O-glycosylation cluster encoded by the genes cj1321-cj1326[6]. Cj1321-cj1326-negative strains originate mostly from asymptomatic carriers and the environment. Thus, flagellin O-glycosylation may play as well a role in cell invasion, and in consequence for the virulence in humans.

Another study of Feodoroff and coworkers identified a C. jejuni-subpopulation in which they were able to detect the gamma-glytamyl-transpeptidase gene (ggt) but not the fucose permease gene (fucP), the phospholipase A gene (pldA) and the enterochelin-uptake-binding-protein gene (ceuE) using pldA- and ceuE-primers derived from the NCTC 11168 genome sequence (The corresponding genes are designated in the following as pldA11168 and ceuE11168) [7]. These isolates could be associated with a higher rate of hospitalizations and bloody diarrhea [7].

To determine the distribution of these further genetic markers as well as their association with ansB, dmsA,ggt, cj1585c, cj1365c and dimeric tlp7 and secondary their correlation with the clinical data of the above mentioned studies, we further characterized the same 266 isolates by screening for the presence of eight additional genetic markers: the flagellin O-glycosylation locus cj1321-cj1326[6], the L-fucose permease gene fucP[8], the outer membrane siderophore receptor cj0178[9,10], the iron uptake protein/ferric receptor cj0755/cfrA[9,10], the enterochelin uptake binding protein ceuE[11], the outer membrane phospholipase A pldA[12], as well as the lipooligosaccharide sialyltransferases cstII and cstIII[13,14].

Results

The frequency of all eight new determined genetic markers in all tested 266 isolates and in each subgroup is listed in Table1. Additionally the ratio of human isolates as parameter for the clinical relevance of the particular isolate group is listed there. A pictorial representation of the marker gene distribution among the various subgroups as well as their isolate origin is shown in Figure1.

Table 1

Distribution and association of genetic markers, LLC and MLST-CC within the determined subgroups

(sub-) group	No. of isolates with marker gene/total no. (%)									human origin
	cj1321-1326	fucP	cj0178	cj0755	ceuE111681	pldA111682	cstII	cstIII	LLC3
1a	38/38#(100)	38/38#(100)	38/38#(100)	38/38#(100)	38/38#(100)	38/38#(100)	13/38°(34.2)	33/38#(86.4)	C/A	16/38(42.1)
1b*	43/44#(97.7)	44/44#(100)	44/44#(100)	44/44#(100)	42/44°(95.5)	41/44(93.2)	16/44°(36.4)	37/44#(84.1)	C/A/B	19/44(43.2)
1b**	38/38#(100)	36/38#(94.7)	37/38#(97.4)	38/38#(100)	35/38(92.1)	37/38°(97.4)	37/38#(97.4)	2/38#(5.3)	B2	19/38(50.0)
1b***	7/15(46.7)	5/15°(33.3)	15/15#(100)	15/15#(100)	14/15#(93.3)	15/15#(100)	6/1z(40.0)	0/15#(0.0)	B, D	9/15(60.0)
2a	2/17#(11.8)	0/17#(0.0)	0/17#(0.0)	3/17#(0.0)	12/17(70.6)	14/17(82.4)	16/17#(94.1)	1/17#(5.9)	A1/B	8/17(47.1)
2b	3/34#(8.8)	1/34#(2.9)	1/34#(2.9)	1/34#(2.9)	26/34°(76.5)	29/34(85.3)	5/34#(14.7)	0/34#(0.0)	D/E/H/U	22/34°(64.7)
3a*	15/22(68.2)	18/22°(81.8)	22/22#(100)	22/22#(100)	18/22(81.8)	18/22(81.8)	18/22#(81.8)	1/22#(4.5)	-	15/22°(68.2)
3a**	16/19°(84.2)	2/19#(10.5)	19/19#(100)	19/19#(100)	18/19#(94.7)	11/19(57.9)	12/19(63.2)	7/19(36.8)	E	4/19°(21.1)
3b	2/11°(18.2)	0/11#(0.0)	11/11#(100)	11/11#(100)	10/11(90.9)	8/11(72.7)	10/11(90.9)	1/11(9.1)	-	3/11(27.3)
4	3/8(37.5)	0/8#(0.0)	1/8#(12.5)	0/8#(0.0)	7/8(87.5)	6/8(75.0)	5/8(62.5)	0/8#(0.0)	-	2/8(25.0)
5	0/4#(0.0)	1/4(25.0)	4/4#(100)	4/4#(100)	4/4#(100)	4/4#(100)	2/4(50.0)	0/4#(0.0)	-	1/4(25.0)
6	3/9(33.3)	9/9#(100)	9/9#(100)	9/9#(100)	8/9(88.8)	8/9(88.8)	2/9°(22.2)	0/9#(0.0)	A/D	7/9(77.8)
all	170/266(63.9)	154/266(57.9)	204/266(76.7)	208/266(78.2)	232/266(87.2)	229/266(86.1)	142/266(53.4)	82/266(30.8)	all	128/266(48.1)

Marker genescjj1321-cj1326:O-linked flagellin glycosylation locus; fucP: L-fucose permease gene (cj0486); cj0178: outer membrane siderophore receptor; cj0755: iron uptake protein (ferric receptor cfrA); ceuE: enterochelin uptake binding protein; pldA: outer membrane phospholipase A; cstII: LOS sialyltransferase II; cstIII: LOS sialyltransferase III; LLC: lipooligosaccharid (LOS) locus class; MLST-CC: Multilocus sequence typing clonal complex; footnotes: 1negative corresponds to only detectable using the forward primer based on the 81-176 genome sequence: 5’-GAT-AGA-GTC-GCA-GGC-GTT-CC-3’+2negative corresponds to only detectable using the forward primer based on the 81-176 genome sequence: 5’-AAA-CTT-ATG-CGT-TTT-T-3’ 3LLC according to Habib et al. 2009 [3], Hotter et al. 2010 [15], Revez et al. 2011 [16]; p<0.05/# p<0.001 significance level in comparison to the remaining isolates belonging not to the corresponding group, additionally the values in subgroups with above average numbers of positive isolates are given in bold numbers; in the case of ceuE and pldA the NCTC 11168 typical allele presence is given in bold if the isolate numbers were above average.

Figure 1

MLST-sequence based UPGMA-tree and the arrangement of the six different marker genes within the six defined groups (twelve subgroups). On the left side the MLST-sequence based UPGMA-tree of 266 C. jejuni isolates is depicted. The numbers shown on the branches of the tree indicate the linkage distances. The right side of the table lists all isolates in the order of the UPGMA-tree depicting the source of the isolate, the presence or absence of the six marker genes and their belonging to one of the groups listed in Table1. Source: Human isolates are marked blue, chicken isolates yellow, bovine isolates red, and turkey isolates green. Marker genes: Presence of a genetic marker is marked with a light red shade, absence with a light green shade. The marker genes from left to right are: cjj1321-6:O-linked flagellin glycosylation locus; fucP: L-fucose permease gene (cj0486); cj0178: outer membrane siderophore receptor; cj0755: iron uptake protein (ferric receptor cfrA); ceuE: enterochelin uptake binding protein; pldA: outer membrane phospholipase A; cstII: LOS sialyltransferase II; cstIII: LOS sialyltransferase III; The last column gives the group according to Table1: light grey (1A), light yellow (1B*) intense yellow (1B**), dark yellow (1B***) cyan blue (2A), bondi blue (2B), carrot-orange (3A*), orange-red (3A**); rust-red (3B), turquoise [4], red [5], steel-blue [6] and white (singeltons).

The flagellin O-glycosylation locus cj1321-cj1326 as marker for livestock-associated strains could be detected in the majority of the isolate groups: 1A, 1B*, 1B**, 3A and 4, assuming their livestock association. In contrast to that, especially the groups 2A + B as well as 1B***, 3B and 5 were negative for this marker gene.

A comparable distribution pattern could be demonstrated for the fucP gene. The isolate groups 1A, 1B*, 1B**, 3A* and 6, are positive for this marker gene, whereas the fucP genes was nearly absent in the groups 1B***, 2A + B, 3A** + B and 4.

Feodoroff and coworkers identified a subpopulation in which they were not able to detect ceuE using ceuE-primers derived from the NCTC 11168 genome sequence [7]. The same phenomenon was described by them for pldA using NCTC 11168 genome based primers, but here the differences were not significant [7]. Using additional forward primers based on the gnome sequence of the 81–176 strain (see Table2), we could detect ceuE and pldA in the whole test population. Using exclusively the NCTC 11168 genome based primers a significant lowered ceuE-detection rate was only observerd for group 2 isolates (24.0%, p < 0.002). There were no significant differences in the pldA detection using additional 81–176 genome-based primes in our study population.

Table 2

Primer

Gene	Primer name	Sequence 5’-3’	Annealing temp	Reference
cj0178	cj0178-F01	TGTAGGCGGGGGTGGCAAGA	54.0°C	this study
	cj0178-R01	ACGACCGCGAGCAGAATTGC
cj0755/cfrA	cj0755/cfrA-F01	ATGGCCGCGAAGTCGTAGGG	54.0°C	this study
	cj0755/cfrA-R01	AGCGATCTATTTGCCACTCGCCT
cj1321	CjNCTC11168-1321_f	AAAATGTCATCATCATAGGAGCG	60.0°C	[6]
	CjNCTC11168-1321_r	TCTAAGTTTACGCAAGGCAACA
cj1322	CjNCTC11168-1322_f	GACTTTGGTTTAATGGGTAAGCA	59.6°C	[6]
	CjNCTC11168-1322_r	TTCCGGCGTTAAAATTAGAAAA
cj1323	CjNCTC11168-1323_f	AGAACGATTTACCCCATTGAAA	59.7°C	[6]
	CjNCTC11168-1323_r	ATTTGCTAAAGCTCCTCGATTG
cj1324	CjNCTC11168-1324_f	TGCCGTAAGTGGAGGTAAAGAT	60.0°C	[6]
	CjNCTC11168-1324_r	TCTGCACACATTGTTCTATCCC
cj1325	CjNCTC11168-1325_f	ACGGATTACTTTTTCCAGATGGT	60.0°C	[6]
	CjNCTC11168-1325_r	TTTGCTTTGAAAATACGCTGAA
cj1326	CjNCTC11168-1326_f	TACATTTCATCGATAAAGCCGA	59.7°C	[6]
	CjNCTC11168-1326_r	AAATATAATGGTGTGCCGATCC
fucP	cj0486FWD	GATAGAGCATTAAATTGGGATG	52.0°C	[8]
	cj0486REV	CCTATAAAGCCATACCAAGCC
	rpoC	GAACTTGCTATTGCTGAGCC
	rpsL	ACCCTAGTGCAAACTCCCCT
ceuE	ceuE-81176F01	GATAGAGTCGCAGGCGTTCC	60°C	this study
	ceuE405F	GATAAAGTCGTTGGCGTTCC		[7]
	ceuE405R	GCGAGATTGGAGGACCAAAGG
pldA	pldA-81178F01	AAACTTATGCGTTTTT	45°C	this study
	pldA-84fwd	AAGCTTATGCGTTTTT		[7]
	pld-981rev	TATAAGGCTTTCTCCA
cstII	orf7ab	ACTACACTTTAAAACATTTAATCC AAAATCA	56°C	[14]
	orf7ab	CCATAAGCCTCACTAGAAGGTATGAGTATA
cstIII	orf7c	TTGAAGATAGATATTTTGTGGGTAAA	56°C	[14]
	orf7c	CTTTAAGTAGTGTTTTATGTCACTTGG

Furthermore, we included the genes cj0178, an outer membrane siderophore receptor, and cj0755, an iron uptake protein (ferric receptor), in the panel of marker genes. The gene products of cj0178 and cj0755 are like enterochelin, CeuE, involved in the microbial iron uptake. Thus, it was, because of their functional association to CeuE, suggestible that they may be associated with bloody diarrhea like ceuE[7] as well. Both genes could be detected, mostly associated with each other, in more than 76% of all isolates. In the groups 2 (A + B) and 4 they are nearly completely absent, whereas about 100% of the remaining groups are positive for both genes.

Additionally, we looked for the presence of cstII and cstIII in order to distinguish isolates with sialylated LOS from isolates with non-sialylated LOS. There are already more detailed studies associating MLST CC with certain LCC [3,15,16] allowing us to associate a particular isolate group with specific LCC only on the basis of the MLST-CC and the information about the absence or presence of cstII and cstIII (see Table1 and Figure1). Group 1A and 1B* were generally tested positive for cstIII. The subgroup named 1B**, which is comprised of CC 48 and CC 206 isolates, is only cstII but not cstIII positive. Isolates from the subgroup 1B*** (CC 49 and CC 446) are partially positive, partially negative for cstII but generally cstIII-negative. All in all, 23 isolates are positive for cstII and cstIII. Most of these double-positive isolates belong to group 1 (87.0%) and CC 21 (65.2%).

The isolates of group 2A are in the majority cstII-positive, in contrast to group 2B isolates that are negative for both, cstII and cstIII, which means that these isolates bear a non-sialylated LOS. Most of the group 3 isolates are positive for cstII but not cstIII, besides a minority of CC 353 isolates that are cstIII-positive. The majority of isolates in the groups 4, 5, and 6 are cstII- and cstIII-negative (non-sialylated LOS).

Finally the ratio of human isolates in comparison to all animal isolates was significantly (p = 0.04355) increased in the ggt-positive subgroup 2B, whereas the difference for the whole group 2 (A + B) was increased but not significant. An increased ratio of human isolates could be also detected for the fucP-negative subpopulation (p(1B*** + 2) = 0.04790) as well as the ceuE-negative (referring to a PCR using NCTC 11168-based primers) subpopulation (p(2 + 3A*) = 0.00825). However, we could not detect any significant association between a particular animal host species and the presence of the eight tested genetic markers (results not shown). With the exception of group 1B** with a significant (p = 0.01374) lower hospitalization rate and group 3A* with a significant (p = 0.00020) lower rate of bloody diarrhea no significant differences in the clinical parameters could be detected within this study population.

Discussion

Looking at all detected genetic markers we could describe two major types of marker gene combinations represented by group 1A and group 2B. All other groups depict a gradual transition of marker gene combinations between these two groups. Thus the main focus on attention should be on these two groups. Group 1A is characterized by the presence of cj1365c, cj1585c, dimeric tlp7[2], cj1321- cj1326, fucP, cj0178, cfrA/cj755, and ceuE as well as the absence of ansB, dmsA, ggt and cstII. In contrast to that, group 2B is an inverted mirror image of this constellation: positive for ansB, dmsA, ggt but negative for cj1365c, cj1585c, dimeric tlp7[2], cj1321- cj1326, fucP, cj0178, cfrA/cj755, ceuE as well as cstII/III.

Champion and coworkers identified the flagellin O-glycosylation locus cj1321-cj1326 as marker present in livestock-associated strains, whereas 55.7% of clinical isolates were shown by them to be negative for this gene cluster [6]. According to their data, cj1321-cj1326-negative strains originate mostly from asymptomatic carriers and the environment [6]. Due to our data, 63.9% of the tested C. jejuni isolates show livestock association based on the presence of cj1321-cj1326. But in contrast to their findings the non-livestock-associated group 2B is significantly more often associated with human origin and thus, bears obviously higher pathogenic potential for humans than the livestock-marker positive strains.

The fucP gene was shown to be present only in isolates negative for ggt[8], which is in accordance with our findings. The ggt-positive group 2 is almost completely free of fucP-positive isolates. Interestingly, group 6 isolates, positive for the ggt-associated marker genes ansB and dmsA but not for ggt, are mostly able to utilize L-fucose. The fucP distribution pattern is similar to that of the livestock-association marker genes cj1321-cj1326 and the serine protease Cj1365 [2]. Thus, fucP should be considered as a further marker for livestock association. It can be suggested that the fucose permease is a crucial prerequisite for dwelling in the mucosa layer, while it enables the bacterial cell to metabolize mucosal L-fucose.

The ability to acquire iron is an essential prerequisite for bacterial replication and thus an important virulence factor especially in iron restricted environments [17,18]. While C. jejuni has no own siderophores [10] it makes use of exogenous siderophores produced by accompanying bacterial species [19]. At all five different iron uptake systems have been detected in the genome of C. jejuni NCTC 11168 [10], but the genome sequence of strain 81–176 reveals three fundamental differences in this regard [9]. Cju15, a protein of unknown function, replaces the gene cfrA/cj0755, which encodes a ferric uptake receptor [9]. A second iron uptake transport system encoded by the genes cj0173c-cj0182 is missing critical components e.g. cj0178 and tonB3[9], and in the gene cluster encoding the enterochelin uptake system cju30 is inserted between cj1355 and cj1356c[9]. Additionally the enterochelin uptake system (CeuBCDE; Cj1352 to Cj1355) is ubiquitous within the C. jejuni population, but it shows sequence variability detectable by PCR using different primers. A C. jejuni subpopulation, associated with a higher rate of bloody diarrhea requiring hospitalization, was identified by Feodoroff and coworkers [7]. This subpopulation was positive for ggt, but ceuE was not detectable using ceuE-primers derived from the NCTC 11168 genome sequence. This subpopulation corresponds to group 2 in our scheme. In a significant number of group 2 isolates it was only possible to detect the ubiquitous gene for ceuE using primers derived from the genome sequence of C. jejuni strain 81–176 (for pldA we detected no significant differences). In this group of isolates the iron uptake system components cj0178 and cfrA/cj755 are absent in nearly 100% of the isolates. Thus, the two groups identified by Feodoroff et al. associated with bloody stools/GGT-production and an increased hospitalization rate/ceuE11168-presence overlap to a larger part that corresponds to group 2B. Besides ggt and ceuE11168, cj0178 and cfrA/cj755 should be considered as marker genes correlating with clinical data.

Parker et al. defined, according to the organization of the LOS locus, various LOS locus classes (LLC). The LOS locus of LLC A, B, C, M and R includes the sialic acid synthase (neuBCA) and two class-specific sialyltransferases: cstII in LLC A, B, M, R and cstIII in LLC C [19,20]. It was demonstrated that the LOS plays a role for epithelial cell invasion [4] and is associated with the clinical course of gastro-enteritis [5]. In this study, we detected just the key-enzymes for LOS sialylization cstII and cstIII. Besides the isolates of the groups 2B and 6, the test population was either cstII or cstIII positive. Group 1A and 1B* isolates were predominantly positive for cstIII. This corresponds to the results of Habib et al. that CC 21 belongs to either LCC C or LCC A [3]. The subgroup 1B**, consisting of CC 48 and 206 isolates, is only cstII but not cstIII positive, corresponding mostly to LLC B [3,15]. The isolates of the subgroup 1B*** (CC 49 and CC 446) were demonstrated to be partially positive, partially negative for cstII but generally cstIII-negative. This corresponds to LLC B and D due to few isolates described by Habib et al.[3]. The majority of group 2A isolates was tested positive for cstII, corresponding to LCC A1 and B [3,16] in contrast to group 2B isolates that were tested negative for both cstII and cstIII and belong to LLC D and E(H) [3]. Positive tested for cstII but not cstIII was the majority of isolates in group 3. An exclusion were the isolates of CC 353 that are cstIII-positive (corresponding to LCC C). The negative test result for cstII- and cstIII of the majority of isolates in the groups 4, 5, and 6 implies that they belong to LLCs with non-sialylated LOS. Hotter et al. associated LCC D and E, corresponding to group 2B in our study, with an increased hospitalization rate [5], that is in accordance with the results obtained by Feodoroff and coworkers for the ggt-positive and ceuE11168-negative group [6] as well as with our prevalence rates for isolates of human origin. In contrast to our data and the data of Feodoroff et al.[7] Hotter and coworkers associated LCC B and C with a higher frequency of bloody stools [5]. This group of isolates corresponds for the most part to the group 1 but also 2A.

Conclusions

In general, the arrangement of the eight additional marker genes and the ratio of isolates of human origin substantiates and complements our prior definition of the subgroups.

One outstanding population formed by the groups 1A + B, which is able to utilize L-fucose, seems to be livestock-adapted due to the presence of cj1321-cj1326, cj1365c and cstII and/or cstIII, and has all of the five identified putative iron uptake systems of C. jejuni. These strains do not exhibit the genes for an extended amino acid metabolism. Due to their livestock adaptation these isolates are less prevalent in humans and secondarily associated with less severe campylobacteriosis.

Contrary to that, group 2 isolates possess an extended amino acid metabolism (positive for ansB, dmsA, as well ggt) and are not able to metabolize L-fucose (fucP-negative). Group 2 isolates possess only three of five iron uptake systems. This group splits into the two subgroups 2A and 2B. The subgroup 2B is additionally negative for the livestock markers cj1365c, cj1321- cj1326, as well as cstII/III. In contrast to that, subgroup 2A is positive for cj1365c and cstII, but cj1321- cj1326 is likewise not present. Additionally, subgroup 2A is characterized by the presence of the flagellum-secreted nonflagellar protein A1 encoded by fspA1[20]. The remaining subgroups demonstrate a somewhat intermediate marker gene profile compared to 1A and 2B. In this respect, group 6 seems noteworthy, as the corresponding isolates are positive for ansB and dmsA, typical for group 2 as well as fucP, cj0178, cj0755 and cj1365c typical for group 1 but not ggt or cj1321- cj1326. Furthermore, only half of group 6 isolates posses a sialylated LOS.

The high virulent isolate subpopulations identified by Mortensen, who associated LCC D and E with a higher hospitalization rate [5] and these of Feodoroff, who associated ggt and a ceuE gene, that is not detectable with primers based on the NCTC 11168 sequence, with severe campylobacteriosis and bloody diarrhea [7], seem to overlap at least partially in group 2, with the highest pathogenic potential i.e. the highest virulence for humans. Surprisingly, the asymptomatic colonizers identified by Champion et al.[6] and isolates bearing a non-sialylated LOS seem to predominate this high virulent isolate group.

Finally, it should be questioned especially for cstII/III, if there is a causal relationship between a particular genetic marker and clinical parameters, while particular genetic markers are associated with each other and the causal relationship to clinical parameters could be due to a causal relation of an associated genetic marker.

Methods

C. jejuni isolates

A total of 266 C. jejuni isolates, 128 of human, 66 of chicken, 45 of bovine, and 27 of turkey origin, with already determined MLS-type and characterized for six genetic markers were selected from our collection [2]. That means about half of the isolates were of human (128) and half of animal (138) origin, what should help to make statements about the clinical relevance of a particular isolate group due to the proportion of isolates originating from human stool samples. The avian and bovine isolates were obtained from the German Campylobacter reference center at the Bundesinstitut für Risikobewertung (Federal Institute for Risk Assessment) in Berlin, Germany. The human isolates originate from stool samples of hospitalized patients of the University Medical Center Göttingen, Germany (40%) as well as outpatients of several doctor’s offices in the city of Göttingen (60%). For these strains the parameters watery diarrhea (85%) vs. bloody diarrhea (15%) are known. Additionally 42 well-characterized isolates of the CampyNet research network strain collection were included as references. All isolates of this study were PCR-positive for ciaB and the cdtB.

The C. jejuni isolates were cultured on Columbia agar base (Merck) supplemented with 5% sheep blood (BA) and incubated at 42°C under microaerophilic conditions (5% O2, 10% CO2, 85% N2) for 24 hours prior to DNA extraction.

DNA extraction and marker gene detection

Genomic DNA of C. jejuni was isolated using the QIAamp DNA Mini Kit (Qiagen) according to the manufacturer’s instructions. For detection of the different genetic markers the primers listed in Table2 were used.

Phylogenetic analysis

For construction of a UPGMA-dendrogram (unweighted-pair group method using average linkages) the MEGA4 software was used [21], and the C. jejuni MLST website (http://pubmlst.org/campylobacter/) developed by Keith Jolley and Man-Suen Chan, sited at the University of Oxford was consulted for assignation of sequence types and clonal complexes [22].

Statistical analyses

Statistical analysis was performed using the Statistica software. The χ²-test was used to test for significant differences/similarities in the frequencies of the various genetic markers within the defined groups. The obtained p-values are indicated in Table1.

Abbreviations

GBS: Guillain-Barré-syndrome; LOS: lipoologosaccharide; LLC: lipoologosaccharide locus classes; ggt: gamma-glytamyl transpeptidase gene; ceuE: enterochelin uptake binding protein; ciaB: Campylobacter invasion antigen B gene; cdtB: cytolethal distending toxin subunit B gene; cj: gene numbering based on the genome sequence of Campylobacter jejuni strain NCTC 11168; cfrA: ferric receptor gene in C jejuni (iron uptake protein); fucP: L-fucose permease gene; pldA: outer membrane phospholipase A gene; cstII/III: lipooligosaccharide sialyltransferases II and III genes; ansB: asparaginase gene with an N-terminal sec-dependent secretion signal; dmsA: dimethyl sulfoxide oxidoreductase subunit A gene; tlp7: transducer like protein 7 gene; UPGMA: unweighted-pair group method using average linkages; MLST: multi-locus sequence typing; CC: clonal complex.

Competing interests

All authors declare no competing interests.

Authors’ contributions

AEZ conceived the study idea, performed all mathematical analysis and drafted the manuscript, CO performed bacterial culture, DNA isolation and PCR-analysis, AMT performed DNA isolation and MLST-PCR, RL performed DNA sequencing and assisted in drafting the manuscript. UG participated in the study design and helped drafting the manuscript. All authors read, commented and approved the manuscript.