key: cord-0031621-4d3qfg6p
authors: Igere, Bright E.; Okoh, Anthony I.; Nwodo, Uchechukwu U.
title: Non-serogroup O1/O139 agglutinable Vibrio cholerae: a phylogenetically and genealogically neglected yet emerging potential pathogen of clinical relevance
date: 2022-05-14
journal: Arch Microbiol
DOI: 10.1007/s00203-022-02866-1
sha: 831699092e08db065f35b9bfbb54b88505efd0b0
doc_id: 31621
cord_uid: 4d3qfg6p

Somatic antigen agglutinable type-1/139 Vibrio cholerae (SAAT-1/139-Vc) members or O1/O139 V. cholerae have been described by various investigators as pathogenic due to their increasing virulence potential and production of choleragen. Reported cholera outbreak cases around the world have been associated with these choleragenic V. cholerae with high case fatality affecting various human and animals. These virulent Vibrio members have shown genealogical and phylogenetic relationship with the avirulent somatic antigen non-agglutinable strains of 1/139 V. cholerae (SANAS-1/139- Vc) or O1/O139 non-agglutinating V. cholerae (O1/O139-NAG-Vc). Reports on implication of O1/O139-NAGVc members in most sporadic cholera/cholera-like cases of diarrhea, production of cholera toxin and transmission via consumption and/or contact with contaminated water/seafood are currently on the rise. Some reported sporadic cases of cholera outbreaks and observed change in nature has also been tracable to these non-agglutinable Vibrio members (O1/O139-NAGVc) yet there is a sustained paucity of research interest on the non-agglutinable V. cholerae members. The emergence of fulminating extraintestinal and systemic vibriosis is another aspect of SANAS-1/139- Vc implication which has received low attention in terms of research driven interest. This review addresses the need to appraise and continually expand research based studies on the somatic antigen non-serogroup agglutinable type-1/139 V. cholerae members which are currently prevalent in studies of water bodies, fruits/vegetables, foods and terrestrial environment. Our opinion is amassed from interest in integrated surveillance studies, management/control of cholera outbreaks as well as diarrhea and other disease-related cases both in the rural, suburban and urban metropolis.

Cholera has been listed amongst tropical disease which occurs from infection by pathogenic microorganisms whose members are grouped as enterobacteriaceae. This family houses pathogens which are implicated in systemic Vibriosis, diarrhea and diarrhea-like symptoms as it infects both intestinal tissue and enterocytes. The tissue/enterocyte infecting pathogenic family of organism is grouped taxonomically as Vibrionacea members. According to the Bergeys manual of Systematic Bacteriology (Garrity et al. 2005; George et al. 2005) , the family of Vibrionaceae is made up of 44 known species. Amongst them, 12 are implicated in human diseases including neonatal meningitis, septicaemia, diarrhea and/or wound infections (Igere et al. 2022; Lu et al. 2014; Farmer et al. 2003) . This family (Vibrionaceae) is classified under the eleventh Vibrionales Communicated by Erko Stackebrandt. order and their members are known opportunistic pathogens of animals. Other characteristics common to its members includes free living chemohetrotrophs, marine commensal which play the role of nutrient regeneration, biogeochemical cycling, and biodegradation, etc. (Peng et al. 2021; Wang et al. 2021) . V. cholerae is a member of the family Vibrionaceae which has shown high variability especially amongst successive outbreaks or occurrence. Its existence and endemic/pandemic status in habitats depend on the presence of environmental reservoir strain especially if such environment is employing high sanitary and public hygienic procedures (Ramirez et al. 2021; Brehem et al. 2021) . In poor sanitary environment, their endemic/pandemic level depends on a transient strain or transit type which may have been carried to such environment ). It has a high global distribution and density in Coastal water bodies (Morris et al. 2018) . Some of its members do not carry the gene type for cholera disease (choleragen) while others do. Based on the cell wall polysaccharide component type of these pathogens, they are categorized into two serogroups which are the somatic antigen agglutinating type (SAAT) or O1/O139 V. cholerae while the second group is the somatic antigen non-agglutinating strains type-1/139 V. choleraee . This division into two sero-group members are based on some characteristic features possess by some members. Whereas some strains habour in their cell surface polysaccharide, a particular antigenic determinant called the somatic antigen, others somatic antigen differs due to mutation on their somatic antigenic genelocus (Aydanian et al. 2011) . These antigenic determinants are defined on the basics of bacterial surface antigens categorized as, somatic (O), flagellar (F) and capsular (K), which are associated with the Vibrio lipo-polysaccharide extracellular or surface capsule and flagellum, respectively (Aydanian et al. 2011; Farmer et al. 2011) . The somatic antigen is represented by the alphabet 'O' while the numbers preceding the alphabets indicates the case period of isolation or detection (from first to the last). The numbers preceding the alphabets may also be associated with the pathogenic potential and the relative implication of the potential pathogen in outbreak cases. Clinically, the O1/O139 V. cholerae has been reported as the pathogen of increased relevance as it is involve in most documented cholera cases in the world today (Momba and Azab El-Liethy 2017; Rao and Surendran 2010) . The World Health Organisation further affirmed that major cholera reported outbreak cases are implicated by the sero-group O1, and O139 members (WHO 2014; . However, the other members (O2, O6, O10, O12, O14, O37, O75, O141 etc.) are referred to as somatic antigen type-1/139 non-agglutinable strains (SANAS-1/139-Vc or nonserogoup agglutinating O1/O139 V. cholerae (NSA-O1/139Vc) (Chatterjee et al. 2011; Sack et al. 2003) . The SANAS-1/139-Vc member does not possess cell surface polysaccharide and antigenic determinant for agglutinating somatic antgen type-1/139 as the name specifies, yet its members (V. cholerae strains) (Shan et al. 2022; Devi et al. 2022; Malayil et al. 2011) may be implicated in cholera outbreak case, wound, septicemia, gastro-enteritis and diarrhea. These Vibrio members have been in existence in the environment (water, plankton/sediment and fishes) since the discovery of the family Vibrionaceae in 1890 . According to various investigators and researchers in the area of vibriology, the non-serogoup O1/O139 agglutinating V. cholerae members existed prior to reports on pathogenic or choleragenic Vibrio strains (Faruque et al. 2003) . The NAG members were first reported at Germany in 1896 ). According to the study, somatic antigen non-agglutinable strains (SANAS) were isolated from fishes in the Elbe river of Germany which necessitated their biotype name as "Albensis" . By 1983, a similar isolate of somatic antigen nonagglutinable strain of type-1/139-V. cholerae was isolated from the Santa Cruz Pacific Ocean indicating that the pathogen exist in the environment as a residential microbial flora . V. cholerae Non-O1/Non-O139 strains have been reported in Norway to be implicated in food borne Vibriosis (Rehulka et al. 2015; Bauer et al. 2006) . The European food related disease report data base reveals that in 2005, the consumers of ready-to-eat headless shell fish and black tiger shrimps were observed to pass out diarrhea stool and express other choleragenic Vibriosis symptom (Rehulka et al. 2015; Bauer et al. 2006) . The observation was further confirmed to be associated and implicated with SANAS-type-1/139-V. cholerae. A similar incidence was reported at Denmark in 2008 as the culture of diarrhea stool from consumers of shell fish and shrimps show growth of the NAG Vibrio members (Collin and Rehnstam-Holm, 2011; Halpern et al. 2008 ). This occurrence of SANAS-type-1/139-Vc lasted for almost the same year resulting increased concern amongst clinicians until it was eliminated toward the end of 2008 (ec.europa.eu/food/food/ rapid alert/rasff_portal-database_en.htm). Halpern and his group in 2008 also isolated and detected SANAS-type-1/139-Vc amongst some fishes (Tilapia specie) in Northern Israel fresh water bodies (Halpern et al. 2008) . Other SANAS-type-1/139-Vc strains have also been recovered from fecal specimen of some apparently healthy Tursiops truncates, an Atlantic bottlenose dolphin which was collected from both Florida and Texas (Alphonsa 2013; Buck et al. 2006; Buck and McCarthy, 1994) . It is imperative to note that strains of the NAGVc (generally known as "non-O1/non-O139 V. cholerae") are shown to be: non-choleragenic, non-pathogenic, they are asymptomatic colonizers of human subjects, they are associated with mild and/or sporadic illness (such a gastroenteritis), they are implicated in abrasive tissue infections (wound or ear infections) in apparently healthy individuals (Octavie et al. 2013; Cariri et al. 2010; Morris, et al. 1981) . In immuno-compromised hosts (or those with underlying disease), NAG (non-O1/ non-O139) V. cholerae members are capable of causing exfoliated wound infections, tissue necrosis or sepsis, and high Page 3 of 28 323 mortality (Zmeter et al. 20182017) . Notable example of such members of the NAG Vibrio are O2, O6, O10, O12, O14, O37, O75, O141 etc. as depicted in Table 1 (Crowe et al. 2016; Haley et al. 2014; Aydanian et al. 2011; Tobin-D'Angelo et al. 2008) . It is worthy to note that recent documents from CDC-COVIS-WHO revealed that members of 075 and 0141 which are NAG-O1/O139 have been observed in outbreak cases (WHO 2017; CDC-COVIS 2012) . These reports reveal the need for research based interest/focus/expansion on the nonagglutinating O1/O139 V. cholerae (SANAS-1/139-Vc) pathogen and necessitates an integrated surveillance, control and management strategy for the potential pathogen Table 2 . It is imperative especially in areas/regions of non-documented history of outbreaks or cholera non-endemic regions as previous reports have shown that outbreak of new strains does occur in regions were there are no previous history Fig.1 . In addition, following the trends of previously reported outbreaks, it was shown that only the causal strains are managed/controllled during outbreaks (choleragenic V. cholerae O1/O139) due to its pathogenic relevance in the environment. There is a potential possibility that the source pathogen to an outbreak is masked or a possibility of non-O1/non-O139 pathogen causing a reported outbreak is marsked.

A global improved surveillance scheme, epidemiology and comparative genomics of the pathogen must be initiated and inclusive when considering the management of cholera and cholera-related diseases in both rural, urban, province, country and continent. There have also been a notable underreporting of vibriosis cases globally (Ali et al. 2015) , which may be tracable to discouragement from social, economical, political and societal policy due to the norm that non-O1/ non-O139 are non-pathogenic. Low reporting may also be attributable to limited capacity for epidemiological surveillance and poor work incentives (Ali et al. 2015; WHO 2014; CDC 2010a CDC , b, 2011a CDC , b, 2013 . It is to this end the review was designed to appraise such neglected concern. It also addresses the level of neglect that has greeted research on NAG V. cholerae occurrence, the present situation of cholera in both endemic and non-endemic regions and the involvement of these neglected pathogens in recently observed cases of cholera.

Cholera epidemic has been associated with somatic antigen type-1 (O1) V. cholerae of the classical biotype since the emergence of the disease in 1817. Amongst the 206 and more documented members of the V. cholerae, the Classical biotype of O1 dominated in all cases of cholera until a new biotype was observed as the El Tor. This El Tor type was later displaced in 1992 by a non-O1 serogroup of the somatic antigen which has similar character as the O1 but different in pathotype. Its genes were compared with other somatic antigenic types known (which are O2-O138) as at then but it shows remarkably difference from all existing sero-group types (Faruque et al. 2003) . It was later referred to as O139 V. cholerae which continues to cause epidemic, spreading from India through the entire Asia continent to other continents (Aydanian et al. 2011; Mooi and Bik, 1997; Manning et al. 1995; Nair et al. 1994) . These novel characters observed amongst the O139 members actually change the myth of the Non-O1 involvement in epidemic and choleragenic potential. Some of such characters are acquisition of enterotoxin (CT) and other epidermic associated genes (tcp-gene) (Shan et al. 2022; Faruque et al. 2003; Basu et al. 2000) . From the forgoing, there is a likelihold that the Non-O1 members originated from the O1 V. cholerae members. Early genomic studies observed that the O139 arise from the O1 El Tor member in 1992 which is today classified as the seventh pandemic El Tor Vibrio (7PET) (WHO 2017; Faruque et al. 2003) . According to various investigators, the classification was not based on the detection of the CT gene and tcp gene but other virulence-related genes (WHO 2017; (Faruque et al. 2000) . The study also shows similarity in ribotyping analysis (Faruque et al. 1994 (Faruque et al. , 2000 . In the study of Aydanain and his group, one difference between the O1 and O139 V. cholerae members is the deletion on the gene responsible for the biosynthesis of the somatic antigen in both pathogens (Takahashi et al. 2021; Aydanian et al. 2011 ). This genetic mutation type allows the organism to effect increased virulence and pathogenesis on individual who are previously immune to O1 V. cholerae, hence adults are it's major host. Suffix to say that the somatic antigen carries the epitope for attachment and pathogenicity, hence similar pathogenic effects are expressed amongst O1/O139 members that are agglutinating and other nonagglutinating types (also known as non-O1/non-O139) eg; O5, O2, 04, O27, O37, O53, O65, O75, O141, etc. (Takahashi et al. 2021; Aydanian et al.2011; Tobin-D'Angelo et al. 2008; Nesper et al. 2002; Stine et al. 2000; Yamai et al. 1997) . From the study of Aydanian and his group, it was hypothesized that pathogenic O1/O139 V. cholerae members have the tendency to mutate or change or exchange their somatic antigenic genes which confirms their genetic heterogeneity or plasticity (Aydanian et al. 2011) . This is so, as it ensures escape from preexisting immunity in any reemerging situation of cholera in an environment. This mutation-based activity of O-antigen genes also influence phage lysogeny since somatic antigenic determinants serves as receptor to phage. Other genetic dynamics influenced by the mutation potential of V. cholerae somatic antigenic genes are uptake of free mobile DNA as well as mobile genetic elements (Xu et al. 2013; Blokesch and Schoolnik 2007; Faruque et al. 1998a, b) . The studies of Yamasaki et al. (1999) , Blokesch and Schoolnik (2007) on V. cholerae growth on chitin substrate media also further substantiate serogroup conversion potential. The various genes responsible for somatic antigen were further studied amongst V. cholerae (Samuel and Reeves 2003; Yamasaki et al. 1999) which ensures their classification into different serogroups. These somatic antigenic genes in V. cholerae O1 consists of 18-56 varying units of open reading frames (ORFs) at the lipopolysaccharide subunit (LPS), and consist of sugars and aminoglycosides. Some of these are glucose, fructose and 2,4-Diacetyl-amido-2,4,6-trideoxyglucose (QuiNAc4NAc) which are found in O5 and O8 (Kocharova et al. 2001; Hermansson et al. 1993 ), fucosamine and quinovosamine found in O139 and O108. Other additional subunits are fucosamine (O108), galactosamine (O108), glycero-D-manno-heptose (O5, O8, and O108) and glucosamine (O108) (Kondo et al. 1997) . Hence, the classification of V. cholerae to various serogroup was informed by the subunit sugars and aminoglycosides. The wbf gene regions of these serogroup members also possess high-molecular weight capsules eg O31 and O139 serogroups.

The somatic gene sequence study of V. cholerae by Aydanian et al. (2011) shows that there is 96-100 percent similarity amongst polysaccharide biosynthetic genes. Present also in V. cholerae members LPS is the tendency for gene duplication which suggest a possible future antigenic lineage associated change during epidemic occurrence (Aydanian et al.2011 ).

One of the concerns of non-reporting and negligence in observed disease cases of the Non-O1/Non-O139 V. cholerae, is accessing the genetics of the potential pathogen. Although very few vibriology investigators have reported genetic basics of the potential pathogen, there is paucity of documents that addresses the genetic basis of NSAG/NAG-O1/O139-Vc. The poor research interest/attention given to studies on the V. cholerae non-agglutinationg subgroup after many years of its prevalence reports till the middle of 1980 further emphasized such neglect. Furthermore, following the previous reports from the study of Octavia et al. (2013) , the genomic data of O1 V. cholerae isolates was published which describes some genetic dynamics. They observed about 66 unique sequence types (STs) in their study, three clonal complexities and four subpopulations. The subpopulation I-III are predominantly clinical strains while the subpopulation IV is environmental based. All strains of NSAG/NAG-O1/ O139-Vc were described to belong to four clonal complexity (CC) which are CC1, CC2, CC3 and singleton as interpreted by the eBURST analysis (Octavia et al. 2013) . Amongst all identified NSAG/NAG-O1/O139 V. cholerae members, only the O94 (CC2), O49 (CC3) and O12 (CC3) have different clonal complexity, other members have singleton as their clonal dynamics (Octavia et al. 2013) . The genetics of the Lipopolysaccharide somatic antigen biosynthetic gene of Non-O1 or O139 V. cholerae also shows that it does not possess any side chain in the core LPS while its O1 counterpart possess about 17 side chains of smaller repeated units of 4-NH2-4,6-dideoxymannose. The sub-unit of each O1 member is substituted with the tert-butyl esterified 3-deoxy-L-glycero-tetronic acid, while their major functional gene is wbf which consist of four other genes (gmhD, rjg, orf and manC) (Octavia et al. 2013) .

In 2003, the studies of Chatterjeea and Chaudhuri reported that V. cholerae transfer genes by a P-factor which is not the case with other Gram-negative pathogens (F-factor in other organism). A growing multiple drug resistance was also observed which is associated with R-factor and exclusively traced to plasmid acquisition (Chatterjeea and Chaudhuri 2003). Other genetic basis of the O1/O139 V. cholerae pathogen were also reported by various investigators (Okoh et al. 2014; Octavia et al. 2013; Igbinosa et al. 2009 ), yet there is dearth of research or low documention in reports for non-agglutinating O1-type or O139-type V. cholerae strains. We are of the view that this negligence or under-reporting of these emerging potential pathogens may pose a negative public health impact, affecting management and control negatively especially in disease distribution. It is worthy to note that management/control is said to be plausible when an uncompromised and unreserved attention is given to any suspected source of a problem, hence the need for an unbiased research attention on the SANAS-Vc is reasonable.

Comparative genomic studies, basic genetic relatedness studies and various online data base analysis have shown that all V. cholerae members are closely related as they cluster together indicating that they have a common ancestor/ origin. The phylogenetic study of Rahman et al. (2008) ; Katz et al. (2013) and Aydanian et al. (2015) have shown that all cholera-associated V. cholerae and members that express choleragen tend to cluster closely together. This is related to the associative-concept of the V. cholerae members as having similar "epidemic genotype" which arise from multiple genes implicated in any reported epidemic . A continuous phylogenetic study by other investigators shows that the virulence genes from some non-epidemic associated strain does not cluster with that of V. cholerae members which are usually reported and associated in outbreak cases ). However recent studies show lineage similarity (Aydanian et al. 2015) between SANAS-Vc and the SAAT-Vc. Other atypical cholera cases have been reported to show similar occurrence of diverse unrelated virulent genes among V. cholerae strains, bringing about a debate in the relativity/relationship of the V. cholerae members.

The study of Hasan and his group (Hasan et al. 2012a , b, c) observed a different phylogenetic report after their study on the prevalence and genetic relatedness of Non-O1/Non-O139 or type-O1/O139 non-agglutinating V. cholerae on patients assessed after the Haiti epidemic. A report written to Mekalanos and his group on their observation of differences in phylogenetic deviation was addressed/discussed. Suffix to say that Mekalanos and his group are regular investigators of vibriology. This report sharing was to harmonize the dichotomy in the results generated from various genomic diversity studies (Hasan et al. 2012a, b, c; Mekalanos et al. 2012) , and to interprete the subjects appropriately.

The debate on the relatedness of O1/O139 and Non-O1/ Non-O139 especially as it concerns pathogenic dynamics in outbreak association was then addressed by Hasan and his group. Their report after a reinforced high through-put phylogenetic analysis showed that all clinical isolates of Non-O1/Non-O139 V. cholerae members formed a closely related cluster with clinical isolates of O1/O139 V. cholerae as depicted in a monophyletic clade data which is interpreted as epidemic genotype related (Hasan et al. 2012a, b, c) .

In a comparative study on the genomic island (GI) and pathogenicity island (PI) of NSAG/NAG-O1/O139 V. cholerae and the O1/O139-choleragenic V. cholerae, isolated from Haitian outbreak, it was reported that 18 GIs and PIs were related. A similar study on clinical and environmental isolates revealed 40 similar GIs and PIs genes. This also confirms that both cholera members arise from a single origin. Although there were high GIs and PIs amongst the clinical and environmental isolates, it only indicates possession of additional unidentified fitness factors which may be involve in other virulence indices (Hasan et al. 2012a, b, c) . Other studies also corroborates these reports (Yamasaki et al. 1999; Comstock et al. 1996; Bik et al. 1995; Stroeher et al. 1995; Aydanian et al. 2015) . These reports confirm the genealogical and phylogenetic relationship of both SAAT-1/139-Vc and SANAS/NSAG/NAG-Vc as members of the family Vibrionaceae.

Following the definition of cholera by the Unites State Centre for Disease Control and Prevention (CDCs) in 1996, the clause on "only confirmed cases of cholera be notified" has contributed to the negligence associated with the report on the incidence and/or prevalence of O1/O139-NAG V. cholerae. A confirmed case is such which has received a reproducible and state-of-the-art laboratory analysis for differentiating non-choleragenic situation, cholera-like and choleragenic vibriosis (CDC-COVIS 2011 . Other investigators prefer cholera to be a case if a diarrhea disease can be reproducible by oral ingestion of purified choleratoxin (Mekalanos et al. 2012) . The correctness of these definitions can never be over emphasized, yet it has contributed and welcomed the low-report and/or negligence in reporting all prevalence and incidence results of Non-O1/Non-O139 V. cholerae. It has also necessitated the paucity and research driven interest on the study of 1/139-NSAGVc or Non-O1/ Non-O139 V. cholerae. The Tables 3 and 4 below shows some of the case documents from both environmental and clinical sources but may not have been reported as cases to the appropriate regulatory body eg COVIS.

According to the 2017 document of Centre for Disease Control-Cholera and Other Vibrio Illness Surveillance System (CDC-COVIS 2017) and the National Notifiable Disease Surveillence System (NNDSS), defining/classifying any observed vibriosis case depends on some basic criterials. The COVIS document indicated that probable vibriosis cases must be based on laboratory detection of any specie member of Vibrionaceae (other than the O1/ O139 V. cholerae) from both clinical specimen using culture dependent and culture independent test methods. The document also emphasize that any clinical case which is epidemiologically associated with a basic/supportive laboratory diagnosis indicates a confirmed case criteria and it is also inclusive (CDC-COVIS 2012a, b. In addition, the confirmed vibriosis cases must be such that have shown positive culture dependent diagnosis (using TCBS or VCA or TTGA), serology and/or rapid culture independent diagnostic test (CIDTs) from vomitus or fecal samples.

Such case must include also the non-choleragenic (nontoxigenic) and the choleraegenic (toxigenic) V. cholerae genotypes irrespective of their serogroup, although special attention must be given to the O1 and O139 members. This is so, as the O1 and O139 V. cholerae members are known for epidemic and pandemic situations. Today other members of the previously known non-epidemic and non-pandemic related have shown potential for pandemic and epidemic cases eg O75 and O141 V. cholerae (CDC-COVIS 2014 , hence, studies on Vibrio is case dependent. Case studies of such should separate the SAAT from the SANAS V. cholerae members. Case reports should also include existing cases or new case reports. Vibriosis detection or observation following the basic laboratory detection criteria (as described by CDC) of any non-O1/non-O139 V. cholerae is tagged an existing case when it is always found in two or more specimen collected while a new case is that which has shown polymorphic gene potential from previously isolated and detected strains. Such detected polymorphism should be based on the new strains virulence determinants, plasmid or extra-chromosomal DNA acquisition, integrative conjugative elements (ICE), antibiotic resistant genes, genomic island (GI), phage acquisition, serogroup diversity etc. The new strain or case associated potential pathogen must be isolated from one or more specimens collected which must also be reported to COVIS. Vibriosis implicated by toxigenic or choleragenic O1/O139-NAGVc continues to pose high public health concern to individual in various areas yet there is a sustained neglect in studying the potential pathogens infectivity and control. Choi et al. 2003 Choi et al. 1988 Choi et al. -1998 Necrotised skin lesion Taiwan/NCKU Hospital 75 yrs Ko et al. 1998 Ko et al. 2009 Ko et al. -2014 Acute gastroenteritis stool Taiwan 

Risk associated with cholera cases are based on seven factorial subjects; Food, Occupation, recreational activities, trauma, natural disaster, international or foreign travel and Hobbies. It is imperative to note that these risk determinants as depicted in Table 5 above are specific to the everyday activities of man, animals, plants and the environment. Some reported cases of O1/O139-NAGVc have implicated migration/travel and consumption of contaminated seafood as vehicles of transmission of these emerging pathogens, yet low attention has been given to studies of these Newton et al. 2011 Newton et al. , 2012 . Other recent study from the Asian continent reveals that Non-O1/Non-O139-Vc is linked to 70% of case that resemble cholera. Some refers to such pathogens as the choleragenic Non-O1/Non-O139 V. cholerae since the various symptoms of SAAT V. cholerae infected patients were observed in NAG infected patients (Dutta et al. 2013; Ismail et al. 2012 ). This rare gastroenteritis are today becoming prevalent amongst hospitalized monomicrobic patients of greater than five years of age and a history of non-choleraegenic Vibrio infections (Janda et al. 2015) .

The NSAG/NAG-O1/O139 or Non-O1/Non-O139 V. cholerae members have shown genetic heterogeneity as reported from the REP-PCR, RAPD-PCR, BOX-PCR and ERIC-PCR study of various investigators (Dalusi et al. 2015a, b; Fooladi et al. 2013; Ateba and Mbewe, 2013; Dutta et al. 2013; Waturangi et al. 2012; Chokesajjawatee et al. 2008) . A significant multiplicity of virulent genes has also been reported by various investigators (Gupta et al. 2016; CDC-COVIS 2013 . This is a clear indication that the pathogenesis of the 1/139-SANAS V. cholerae members does not possess a mono-pathogenesis mechanism since their virulent dynamics are multi-facets. As reported by Morris et al. (2018) , Madhusudana and Surendran, (2013) and Lu et al. (2014) , other factors may also enhance their pathogenesis and development to illness in an infected person. Some of such factors include nearness-to or contact with an infected or carrier agent, poor hygienic practice, immune-stability of hosts, and environmental factors. Other investigators have reported the association/relationship of human blood group type with the infectivity and/or pathogenesis of NSAG/NAG-O1/O139 V. cholerae. (Bennett et al. 2015; Janda et al. 2015) . In human, infection and pathogenesis is initiated only after contact with an infected agent or consumption of contaminated food or water. The food or water passes through the stomach acid barrier allowing the organism to colonize the small intestinal epithelium. With the aid of the tcpgene (toxin coregulated pili), it releases its various virulent factors (including enterotoxin CT) through the bacterial outer membrane into the extracellular melius of the small intestine to disrupt active ionic transport in ilia cells. This our aforementioned statement as the potential pathogens emergence shows that it possess the CT and other virulent genes which may be associated with epidemic tendency. Some of the virulence factors are ctxAB (encoding the A and B subunits of CT), zot (encoding zonula occludens toxin), cep (encoding core-encoded pilin), ace (encoding accessory cholera enterotoxin), hap (haemagglutinin protease), orfU (encoding a product of unknown function) etc. The CT also consists of the repetitive sequence (RS) insertion element which directs integration of virulent genes. The core region of the toxin and the RS element makes up the cholera entero toxin (Mekalanos et al. 2010 (Mekalanos et al. , 2012 Li et al. 2003; Hlady and Klontz, 1996; Mekalanos, 1983 ). In addition, the classical and El Tor members of the V. cholerae possess diverse alleles within the rstR gene. A similar gene profile amongst the SAAT-1/139 members isolated from Calcutta shows two variants type of the rstR allele amongst the O139 strain from Calcutta and environmental rstR allele in environmental Non-O1/Non-O139 strains. Because of the variants found within the rstR allele and tendency to possess or harbor prophages (CTXϕ), they are classified/biotyped as classical, Calcutta, ElTor, Bengal and/or environmental phage (Grim et al. 2010; Hsieh et al. 2008; Kimsey et al. 2004) . Other classical virulence genes found in Non-O1/Non-O139 includes HA/P, HlyA, type III secretion system T3SS, type VI secretion system T6SS, NAG-stn and RTX toxin etc. Analysis of a purified HA/P gene isolated from SAAT-1/139 V. cholerae members shows its enterotoxigenic potential in rabbit ileal loop test (RILT). In addition, a heat stable enterotoxin gene (stn/sto) was also detected in the Non-O1/Non-O139 V. cholerae members called NAG-st which also mediate their enterotoxigenic potential (Makri et al. 2007; Purdy et al. 2005 ).

Gastroenteritis This is a disease condition which is associated with passage of watery stool and loss of fluid resulting from the ingestion of a cholera or cholera-like protein/toxin expressing bacterial. Patients with cholera exhibit symptoms of profuse watery diarrhea, vomiting and mild to severe dehydration (Mekalanos et al. 2012) . This is characteristically seen in epidemic cholera cases implicatd by O1 or O139 V. cholerae. Non-O1/Non-O139 V. cholerae which harbours this CT-toxin gene and/or produces similar choleragen seen in most diarrhea cases (Bi et al. 2001 ), but does not possess the epidemic cholera capabilities. It has been reported that some of the O1/O139-NAGVc members tend to habour the epidermic associated genes of V. cholerae O1/O139 in the environment (Zmeter et al. 2018; Baig et al. 2018; Kechker et al. 2017; Engel et al. 2016 ).

This is a bacterial in blood infection which is associated with NSAG/NAG-O1/O139 V. cholerae members, where the infected person does not present any diarrhea or vomiting symptoms as in the case of cholera (Hao et al. 2015) . The pathogen infects blood and meningis of patients resulting remarkable weight loss, increased pulse (about 150 beats/ mins), a temperature of 38-40 °C, abnormal white blood cell count (6.65 × 10 9 L −1 ), 67.1% neutrophils and an elevated level of C-reactive protein (CRP, 88.9 mg/). It will also show a cerebrospinal fluid (CSF) WBC value ranging from 16.65-18.06 × 10 9 with a protein level of 218.6 mg/dl (Schirmeister et al. 2014) . Infants that express such symptoms appear to develop convulsion within 24 h, coagulopathy and metabolic acidosis. A cerebral CT scan of an infected neonate shows that the frontal and temporal lobe possess hemorrhagic focus with symmetric lesions (Hao et al. 2015; Namdari et al. 2000) . Various reported cases of bacteraemia which are implicated by non-O1 V. cholerae infections results increased fatality especially amongst immune-compromised patients (Safrin et al. 1988; Hughes et al. 1978 ). Sharma et al. 1998 ). The symptoms produced by the potential pathogen may in most cases be very severe such that it mimics cholera (Piergentili et al. 1984) . In some cases, the pathogen may be detected in Otitis media (bacterial infection of the ear) as observed by Kechker and his team (Kechker et al. 2017) . In other related cases it is detected in skin lesion or infected liver disease and brain tissue ( Ottaviani et al. 2009 Ottaviani et al. , 2011 Sujatha et al. 2011; Patel et al. 2009; Carvajal et al. 1998 ). Suffice to say that some of the investigators have isolated the potential pathogen from hospitalized patients whose disease case is traceable to contact with various receiving water sheds, creeks as well as other domestic water sources. Table 1 below shows some of the isolated strains/types by various investigators.

Members of the NSAG/NAG-O1/O139 have been shown to thrive mainly in the fresh water environment. The studies of Igbinosa et al. (2009) and Huq et al. (2012) has demonstrated that these Vibrio members are found attached to plankton, plankton associated water bodies, copepod and other zooplankton. Some of them exist in association with sediment, crab, shellfish etc. ). This continuous persistence of the potential pathogen in water bodies as well as domestic water systems may nonetheless generate a negative impact on the management and control of the potential pathogen. It may also have a link with the observed difficulty in the eradication of cholera disease (Okoh et al. 2013; Valdespino and Garcĺa-Garcĺa 2011) in most affected regions. Ceccarelli and his group have observed the prevalence of SANAS-1/139 in water environment with multiple pathogenic dynamics of either pandemic or epidemic relevance (Ceccarelli et al. 2015) . Other vibriologists reported incidence of Non-O1/Non-O139 in plankton, copepod, rotifers, cladocerans and zooplankton (De Magny et al. 2011) . It is envisioned that apart from the incidence of Vibriosis/cholera outbreaks, there is paucity of experimental data/ information to verify prevalence of the SANAS V. cholerae in estuaries and wastewater final effluents. The association of Vibriosis/cholera with flood and other natural disaster is also an epidemiological concern (Bhuyan et al. 2016 ).

The detection of NSAG/NAG-O1/O139 V. cholerae members are subdivided into pathogen differential enumeration, presumptive identification from the environmental and/or clinical specimens using cultural characteristics, biochemical reaction, sugar fermentation, serological delineation and nucleic acid based confirmation using Polymerase Chain Reaction. These combined detection strategies are then divided in four protocols: Culturebased protocol, Serology protocol, biotype protocol and Nucleic acid based protocol which have been standardized overtime (CDC 2015; APHA 2012; ISO 2007) . In outbreak situations, most of these tests should be avoided since a result needs to be confirmed to initiate treatment and report. However, according to Karaolis et al. (2001) and APHA (2012) 

Immuno-diagnostic detection of the SANAS-1/139 V. cholerae members in disease situation remains an unattended area of immediate concern in public health system. This is so, as there is only an applied and borrowed protocol from the parent pathogen V. cholerae O1/O139 due to limited technique, resources and neglect in report of observed cases both in rural, urban and continent alike. Most applied methods are based on reverse or negative detection of O1/ O139 members. Other related detection methods are measurement of vibriocidal antibodies, antibody/antigen agglutination, indirect hemagglutination, reverse passive latex agglutination (RPLA), immunochromatographic test strips and enzyme-linked immunosorbent assay (ELISA) (Yamasaki et al. 2013; Keddy et al. 2013) . Interests are on the rise on rapid detection of the SANAS V. cholerae with a view to determine point-of-occurence cases of the potential pathogen and environmental monitoring/surveillance of V. cholerae. It is to this end that monoclonal fluorescent antibody technique and immunochromatographic dipsticks technique were applied for somatic antigen (LPS subunit) detection and serotyping (Chen et al. 2014; Goel et al. 2005; Nato et al. 2003) . Further immunoassay techniques such as immunofluorescent-aggregation assay (IFAGA) were also designed for the detection of O1 and O139 V. cholerae in water bodies and the environment but not the non-O1/non-O139 V. cholerae members.

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It employs the isolation in a selective media and standard bacteriological determination procedures.

Standard Microbiological methods are being employed to a great extent in the isolation of the SANAS-1/139 members. As documented by Huq et al. (2012) , standard must be ensured when isolating Vibrio cholerae from environmental and domestic water samples. This standard includes collection of water (source), plankton and plankton associated specimen in other to isolate a representative organism in nature from its immediate environment. These water specimen are processed by culturing onto any of Thiosulfate Citrate Bile-salts sucrose (TCBS) agar plates or Vibrio CHROMagar (VCA) or Tellurite taurocholate gelatin agar (TTGA) plates and incubate at 37 °C (Eddabra et al. 2011) . It was also reported that there is need to subject specimen to varying culture techniques and incubation temperature. To enumerate presumptive pathogens, specimen is subjected to membrane filtration technique and 0.20 or 0.45 µm pore size filter membrane is cultured onto freshly prepared TCBS agar or orderwise and incubated at 37 °C for 24-48 h. Observed yellow culture growth are then purified and inoculated onto 20% glycerol stock and stored at -80 °C. Other post detection study may include subjection to a battery of biochemical reaction and sugar fermentation (Cowan and Steel 1974) . Afterwards, the pure colonies are then subjected to an agglutination or serological test. The SANAS does not agglutinate with the somatic antisera (type-1 or type-139), hence it is selected as non-O1 and non-O139. The CDC (2014) Dalsgaard et al. 2001) . Non O1/Non-O139 V.cholerae members were initially after identification reported as causative agent of both small outbreaks relative cases and sporadic cases of cholera-like disease (Okada et al. 2014; Bhattachaiya et al. 2006; Klontz 1990; Morris et al. 1990 ). Other isolates of SANAS V. cholerae which belongs to higher numerical serogroups apart from O1 and O139 does not habour the cholera-related toxin gene (ctx) and the toxin co-regulated pilli (tcp). Hence some of these strains are not accessed and/or reported during outbreak related studies or updated surveillance studies. The relevance of such SANAS V. cholerae members which are neglected due to their presumed non-possession of virulent dynamics should also be assessed both those strains of clinical relevance, environmental relevance and industrial relevance alike.

Specimen of clinical sources should be analyzed after an appropriate observation and cross-examination of some suspected/expected diarrheogenic symptoms. Although, according to Blake and Weaver (1980) , members of NSAG/NAG-O1/O139 V. cholerae and other related organisms, which do not have any epidemic/pandemic-related potential, should not be analyzed. Suffice to say that such symptoms are perculiar with NAG-O1/O139 V. cholerae infections. Others may include mucus stools formation, abdominal cramps initiation, severe to mild fever depending on the immune-competence of the individual, blood type, etc. (Luo et al. 2013) .

Unlike the agglutinative strains of O1/O139 Vibrio members, the NSAG/NAG-O1/O139 Vibrio strains are regularly implicated in most invasive diseases (eg; septicaemia) especially amongst immune-compromised patients (Luo et al. 2013; Rao and Surendran 2010; Lin et al. 1996) . The specimen (fecal/stool, wound swab, exudates) are culture onto specialized selective media and cultures of positive growth are purified and stored as described earlier. According to Luo et al. (2013) , No. 4 Agar may be used for isolation of clinical pathogens since it consists of additional inhibitory agents of clinical diagnostic relevance eg 0.003% rivano powder, 1% sodium citrate, 500 μg/L gentamicin, 0.2% sodium sulphite, 0.5% pig gall powder, 0.1% sodium lauryl sulphate, 0.001% potassium tellurite. It is also of specific note that not all clinical specimen habours choleragenic/toxigenic strains of O1/O139 V. cholerae and/or the toxigenic strains of NSAG/ NAG-O1/O139 V. cholerae. Some of such clinical specimen may also habour non-toxigenic strains. In a similar manner, the environment may also habour both toxigenic/choleragenic and non-toxigenic/non-choleragenic strains. Most reported human clinical cases of Vibriosis associated with NSAG/NAG-O1/O139 clearly show that disease is initiated from ingestion of contaminated food material as well as sea food (Madhusudana and Surendran 2013) . Other sources of contamination include domesticated use of contaminated environmental water, contact with carrier agents and consumption of contaminated shell fish (Rao 2015; Rao and Surendran 2010). In both clinical and environment sources, O1/O139 V. cholerae implication in infection cases has far been reported than cases of NSAG/NAG-O1/O139 V. cholerae members (CDC-COVIS 2017; Kaysner et al. 1987; Baumann et al. 1984) . The study of various early investigators from countries such as Italy has shown high prevalence of other Non-O1/Non-O139 Vibrio strains (eg: O2, O6 O8, O40, O41, O64, and O107 and O158), with negative cholera toxin gene (Filetici et al. 1997) . The situation today appears to differ as current reports shows that Non-O1/Non-O139 Vibrio members are positive to cholera toxin (Kechker et al. 2017; Ceccarelli et al. 2015; Dutta et al. 2013; CDC, 2012; Hasan et al. 2012a,b) . In addition, various strains have also been characterized as NSAG/NAG-O1/O139 V. cholerae, as some either lack the classical virulence determinants or possess the specific virulence factors. These strains include 

Till date, there are no specific Nucleic acid-based techniques applied for the detection of any member of the Non-O1/Non-O139 V. cholerae. Known procedures depend on the negative results from the O1 and O139 detection in both clinical and environmental samples. Although such procedures have survived the taste of time in terms of high sensitivity, specificity, and speed, it is based only on the detection of V. cholerae and the O1/O139 serogroups which use the conventional polymerase chain reaction (PCR) and/or quantitative real-time PCR (Wang et al. 2007; Tebbs et al. 2011; Teklehaimanot et al. 2014; Rao 2015) . The technique detects O1/O139 V. cholerae strains using 16S rRNA, specific gene for detection of the pathogen using the sob gene or the OmpW gene region and agarose electrophoresis of the amplified gene. Other nucleic acid based protocols are nested PCR, duplex PCR and multiplex PCR. Another protocol applied in the separation/detection and diversity study of the cholera toxin is pulsed-field gel electrophoresis (PFGE) (Kong et al. 2002; Tarr et al. 2007; Mendes et al. 2008; Keshav et al. 2010 ). However, nucleic acid based detection and characterization of pathogenic indices including the cholera toxin genes (ctxs) of V. cholerae are being evaluated by numerous investigators (Ceccarelli et al. 2015; Luo et al. 2013; Son et al. 2011; Lipp et al. 2003; Blackstone et al. 2007 ). In the environment, some of these investigators are interested in developing rapid detection methods for the detection of the pathogen. Currently, a developed nucleic acid-sensing dais for choleragenic O1/O139 V. cholerae detection of high specificity and sensitivity is being applied. Such method applies the use of an electrochemical gene sensor and dry reagent or in-silico-based nucleic acid amplification to detect specifically multiple targeted gene of interest (Yu et al. 2015) . This nucleic acid based dais protocol can be harnessed in the detection of other Non-O1 and Non-O139 members of the V. cholerae. Other related hetero-genetic detection of NSAG/NAG-O1/O139 V. cholerae involves virulence or toxigenic/choleragenic genes and in the expression of somatic antigen unidentifiable types or O-untypeable strains (Octavia et al. 2013; Dutta et al. 2013) .

It is important to note that some strains of NSAG 

Restriction Fragment Length Polymorphism which is pronounce riflip or RFLP is a nucleic acid based protocol which detect differences in homologous DNA sequences. It is a technique that employs the digestion of a specimen amplified DNA using known endonuclease or DNA scissor to cut at specific regions of the sampled DNA which eventually produce varying fragments of differential sizes. The cut/ fragmented or restricted DNA specimen is then separated by agarose gel electrophoresis. This method has been applied in various Vibrio studies to delineate closely related biotypes, serogroups and phage-types (Chowdhury et al. 2010; Saha et al. 2006) . It involves the PCR amplification of a specific gene of interest (eg gyrB, tcp, ctxAB etc.) in a specimen extracted DNA and treatment with the endonuclease to fragment into varying/polymorphic sizes. Its banding profile is thereafter detected by electrophoresis and ultra-violet visual system (Urakawa et al. 1997) . This method has been applied in differentiating Vibrionaceae (Urakawa et al. 1997 ) members especially those of high clinical relevance.

Random amplified polymorphic DNA is generally called RAPD which is a nucleic acid based technique that involve amplification of multiple target sites using a short arbitrary single oligonucleotide primer. The primer is synthesized to amplify multiple non-allelic regions of a sampled DNA (Williams et al. 1990 ). The band size profile and differences in amplified region sizes were used to delineate various organisms both at intra or inter specie level and also determine their polymorphism. It has been applied in the polymorphic studies of Vibrio (Sadok et al.2013; Marhual et al.2012; Maiti et al. 2009; Welsh and McClelland 1993) .

The Repetitive Extragenic Palindromic-PCR (REP-PCR) was initially described as regulatory palindromic sequences of untranslated operon regions which is use in epidemiological relationship study. Its applicability is based on the protocol and primers ability to form structures of stable stem-loop in any transcribed or extracted RNA (Higgins et al. 1982) .

It consists of about 38 bp consensus sequence which has six degenerate regions and 5 bp variable loop between the palindromes which are associated with transcription, termination, chromosome organization and mRNA stability (Versalovic et al. 1991; Stern et al. 1984) . This technique has be applied in typing various members of the Vibrionaceae eg V. parahaemolyticus, V. vulnificus,V. alginolyticus etc. (Balcazar et al. 2010; Maluping et al. 2005 Maluping et al. , 2008 Rodriguez et al. 2006 ).

Amplified fragment length polymorphism also called (AFLP) is referred to as another highly sensitive nucleic acid based technique used to identify differences in DNA after treatment with endonuclease. Its basic steps include the use of adaptor complementary primers, extraction of specimen DNA, amplification of DNA, ligation of adaptors to fragmented sticky/blunt ends, amplification of fragments and sequencing of amplified fragments. These fragments are then visualized in a UV-transilluminator or gel documentation system after separation on an agarose gel electrophoresis. Polymorphic genetic elements are then detected from the AFLP profile as relationship and deviation are observed by size of specimen amplified region. The application of this technique in vibriology by various researchers and the discriminating potential of the method has made various investigator to suggest its use in Vibrio studies especially amongst the 7PETs (Mishra et al. 2011; Gomez-Gil et al. 2004; Lan and Reeves 2002; Jiang et al. 2000) .

This is a molecular typing protocol which is based on the application of enteric-bacterial repetitive intergenic consensus oligonucleotide primers for detection of related genes and associated gene patterns. These short primer (126 bp) families are highly conserved sets of oligonucleotide sequences which produce multiple target allele of enterobacterial during PCR amplification. (Bachellier et al. 1999; Hulton et al. 1991) . ERIC-PCR would produce a genetic profile of sampled genomic DNA with regions around ERIC elements and other repeated short DNA sequences. The profile of genetic composition which is produced after electrophoresis may be used to determine relationship and polymorphism amongst sampled DNA. The profile thus produced consists of short base pair regions (126 bp) that appear to be either intergenic regions of polycistronic operons. It's sequences may also appear to be untranslated regions within the open reading frames (Rodriguez et al. 2006) . Some of these regions are novel, homologous and highly conserved nonspecie related hemolysin gene (Hulton et al. 1991) . ERIC-PCR has been successfully applied in the typing of Vibrio species and other bacterial strain (Sawabe et al. 2002; Rivera et al. 1995) . ERIC studies on Vibrio members have shown evident polymorphism in genotypes which is associated with the level of rain fall (Goel and Jiang, 2011) . Other recent reports on the application of ERIC-PCR on V. cholerae also show great diversity in genomic expression. It also indicates a discriminating potential and lesser complexity of ERIC. (Waturangi et al. 2012 ).

BOX AIR elements are multiple, conserved and repetitive DNA sequences which are present in bacterial genome (Gram positive and Gram Negative). There are sometimes referred to as variable number of tandem repeat with sequences that are both specie specific, virulent related and regulatory DNA regions. Earlier reports shows that they were first observed in Gram positive organism (Streptococcus specie) with three specific boxes (Box A, Box B, Box C). Each of the BOX AIR repeat sequence produces specific amplicon size of 59 bp, 45 bp and 50 bp (Linda and Sarita 2014; Sellek et al. 2012; Tulatorn et al. 2018 ) after PCR amplification. These amplicons are produced from the region around BOX AIR element as well as inverted repeat sequences (154 bp) that occur between 12 and 25 amplicons (Tulatorn et al. 2018 ). The profile produced by the primer sequences can be interpreted and applied in the classification of sampled organism and used as a tool in the study of pathogenic dynamism (Ateba and Mbewe 2013). It is used in inter-specie and intra-specie clustering and recently in pathogen source tracking (PST) (Yang and Yen 2012; Johnson et al. 1992a Johnson et al. ,b,c, 2004 . It is also applied in the genealogy of environmental microbes since it is less cost effective and fast in determination with no advance knowledge, negative influence of aged culture and computer assisted methods (Kang and Dunne 2003; Tuang et al. 1999) . Although the technique may be limited in consistency of reproducible results, banding patterns has remained constant (Yang and Yen 2012) . The study of Marques et al. (2008) reported the application of the technique in delineating genomic species of Pseudomonas syringae while other investigators applied in racial differentiation, biovars of Ralstonia solanacearum and typing of Aeromonas members (Tacao et al. 2005; Galal et al. 2003; Paola et al. 1984) . In vibriology, epidemiological relationship of clinical strains and environmental strains are studied amongst choleragenic V. cholerae O1 members (Goel et al. 2010; Kumar et al. 2009; Tulatorn et al. 2018) and other non-cholera Vibrio members (Sellek et al. 2012; Rameshkumar et al. 2011; Gordan 2008; Maluping et al. 2008; Rameshkumar and Nair 2007; Gomez-Gil et al. 2004) . It may also be applicable in the diversity study of SAAT-1/139 members in a polyphasic molecular approach for novel strains.

Although various investigators of Vibrio members have observed and reported numerous cases of V. cholerae occurrence in different estuarine environments, plankton, crab, fish, shellfish, ready-to-eat food stuffs and vegetables, most of their report has shown a high prevalence of Non-O1/Non-O139 V. cholerae in these specimen than the choleragenic O1 Vibrio members (Fri et al. 2017; Deshayes et al. 2015; Trubiano et al. 2014; Yadava et al. 2013; Rashid et al. 2013; Hasan et al. 2012b, c; Kwon 2010) . NSAG/NAG-O1/O139 V. cholerae members have occurred and persisted in various geographical regions as either free living or in association with other organisms such as molluscs, copepod, zooplankton and sponges (Blackwell and Oliver 2008) . Their survival and persistence in the environment are influenced by atmospheric pressure, oxidation reduction potential, temperature, total chlorine, free/residual chlorine and salinity (Owoseni et al. 2017; Beaz-Hidalgo et al. 2010 , Ighinosa et al. 2009 ). Some of these environmental dynamics also ensure its formation of viable but not culturable (VBNC) state, rugose type, smooth types and biofilm formation (Visick 2009; Yildiz and Visick 2009; Asakura et al. 2007; Oliver et al. 2005; De et al. 2004; Islam et al. 2004; Wong and Wang, 2004) . It was also observed that the cholera toxin (CT) and tcp gene were present in some Non-O1/Non-O139 members isolated from the environment which indicated their epidemic causing tendency and ability to cause cholera/ diarrhea/diarrhea-related diseases as well as other extraintestinal infections (Feghali and Adib 2011; Restrepo et al. 2006; Park et al. 2004; Morris and Acheson 2003; Sharma et al. 1998) . This was also previously reported in Calcutta, India by Sharma and his group and recently by Madhusudana and Surendran (2013) . The SANAG-1/139 V. cholerae have been implicated in sporadic epidemic and marine associated infection in crustacean, fishes, shell fish, sediments etc. (Raghul and Bhat 2011; Frans et al. 2011; Ji et al. 2011; Raissy et al. 2011; Soto-Rodriguez et al. 2010; Alagappan et al. 2010; Beaz-Hidalgo et al. 2010; Pal and Das, 2010) . Another area of the SANAG-1/139 V. cholerae studies of salient documentation is their diversity. The diversity of the SANAG-1/139 V. cholerae has also been a concern especially environmental strains which have been reported to be implicated in current human related gastritis, septicaemia, meningitis, wound or soft tissue infection as well as diarrhea (Madhusudana and Surendran 2013) .

Huq and other investigators have pointed that SANAG-1/139 Vibrio association with other environmental organisms (plankton) is noteworthy in the occurrence and their persistence in the environment (Huq et al. 2005; Grossart et al. 2005; Lipp et al. 2003) . Planktons (Phytoplankton and zooplankton) are categorized as marine floating organisms whose products bacterial recognizes, source for livelihood and tends to associate, with a bid to survive within the marine environment (Long et al. 2005; Thompson et al. 2004 ). Planktons may serve as a vehicle for transmission or spread of pathogens as pointed by various investigators (Rehnstam-Holm et al. 2010; Huq et al. 2005 ).

Vibrio cholerae survival in the environment is associated with ability of the flagella to aid movement and adapt in changing environmental situation (Beshiru and Igbinosa, 2018; Odjadjare et al. 2012; Broberg and Calder 2011) . These mobile microbial structures are mainly of two categories which are the polar flagellum and the lateral flagellum. Whilst polar flagella ensures swimming, the lateral flagella alines with other genes for biofilm formation and cellular transformation . Biofilm is a cell-surface associated matrix, it is refered to as a bacterial community were in a bid to survive harsh conditions utilize trapped/ absorbed nutrients to form protective coat using structural genes and regulatory appendages (Yildiz and Visick 2009; Wai et al. 1999) . These genetic appendages are exopolysaccharide biosynthetic gene, lateral flagella and pili gene, c-di-GMP signaling gene, quorum sensing gene and other component regulatory genes (Yildiz and Visick 2009; Snoussi et al. 2008) . This is similar to the characteristics exhibited by Vibrio members as they try to survive enhanced environmental stress, antibacterial and depleted nutrient survival. The activity also favors the inter-relationship of Vibrio members with other bacteria (Yildiz and Visick 2009; Visick 2009 ) as the biosynthesis of exopolysaccharide occurs and flagella/ fimbrial alteration develops to form a three dimensional structure dubbed biofilm (Fong et al. 2010 ). V. cholerae has shown rigid biofilm formation, a characteristic that is traced to its environmental stress survival. Such survival has also be reported to have been facilitated by biofilm formation especially in other Vibrio members (V. parahaemolyticus, V. fischeri and V. alginolyticus) in the environment (Beshiru and Igbinosa 2018; Chavez-Dozal and Nishiguchi 2011) . Currently, Vibrio investigators have purified an antibiofilm activity bioagent (exopolysaccharide A101) from culture supernatant of some marine Vibrio members. Some of its activities act by inhibiting both biofilm formation and distruption of biofilm establishment . Other antibiofilm biomolecule produced is exopolysaccharide QY101, which has similar activity as exopolysaccharide A101. It also eliminate V. cholerae cells from surface material serving as a protection of material and deprivation of Vibrio survival Matz et al. 2005 ).

Regular exposure of Vibrio strains to harsh environmental condition as well as antibiotics has been associated with the incidence of multiple drug resistant strains of SANAG-1/139 V. cholerae. The use of residual chlorine in wastewater treatment facilities and other chemical elements has also been associated with the incidence of drug resistance since bacterial now possess tolerance to chlorine treatment in waste water (Owoseni et al. 2017; Owoseni and Okoh 2017a,b) . Such resistance acquisition is evident amongst NSAG/NAG-O1/O139 V. cholerae members since they are residential floral of the environment and wastewater (Odjadjare et al. 2012) . The study of Chandrasekhar and his group showed that somatic antigen non-agglutinating strains of 1/139 V. cholerae isolated from the environment in Hubli, India are resistant to Fluroquinolone antibiotic members (Chandrasekhar et al. 2008) . A similar antibiotic resistant profile was also found amongst O1 V. cholerae members to ciprofloxacin on isolates from Bangladesh (Kim et al. 2010) . Isolates of NSAG/NAG-O1/O139 or non-O1/non-O139 V. cholerae collected from the Kerala Environment also shows multiple antibiotic resistance at varying degree to various antibiotics eg; nalidixic acid, chloramphenicol, cefotaxime, Streptomycin, trimethoprim, tetracycline, cotrimoxazole, neomycin, ofloxacin, furazolidone, norfloxacin, ciprofloxacin, gentamicin and spectinomycin (Bernard 2006; Jagadeeshan et al. 2009 ). Other multiple antibiotic resistance reported amongst the V. cholerae members were found in the El Tor biotype (Goel et al. 2010 ) which is still increasing.

The clinical, environmental and epidemiological relevance of somatic antigen NAGVc-1/139 or SANAG-1/139 V. cholerae members are today receiving low attention yet reports of its implication in disease cases are on the increase. Various investigators have reported the possible change in the LPS gene structure of V. cholerae members which portend a future association with epidemic outbreaks. Suffice to say that various previous observations have shown that SANAG-1/139 V. cholerae strains possess in their LPS gene structure a tendency for gene duplication which in the future may enhance epidemic and increase pathogenesis. It is also suggestive that future strains associated antigenic lineage may occur as the changing tendency continues in successive outbreak endemic areas. These possible future occurrences pose threat to the management and control of the pathogen if blind research focus and interest is given to the study of the NSAG/NAG-O1/O139 V. cholerae members. The rapid detection of the NSAG/NAG-O1/O139 V. cholerae strains is another area with paucity of reports in vibriology. The reports that the LPS subunits of the somatic antigen consists of sugar and aminoglycosides (such as glucose, glycerol-D-manno-heptose fructose, fucosamine, quinovosamine, galactosamine, glucosamine and 2,4-Diacetyl-amido-2,4,6trideoxyglucose {QuiNAc4NAc}) is another area that has not been harnessed. It has been shown that the serogroup classification of the various NSAG/NAG-O1/O139 Vibrios was informed by the somatic antigen subunit sugars and aminoglycosides. We are optimistic that in the future, if these sugars and aminoglycosides are well studied, a prototype of serogroup antisera for the rapid differentiation of the various NSAG/NAG-O1/O139 V. cholerae members would have been designed and applied. This should be a roadmap to the differentiation and identification of the various serogroup members as well as delineating their pathogenic potential and/or implication in outbreak cases. Other studies on the molecular weight nature of the capsules would also be differentiated using various genetic techniques such as Sodium deodecylSulfate-polyacrylamide gel electrophoresis (SDS-PAGE), thin layer chromatography and subsequent development of chromatogram on a Sephadex LH20. This application would differentiate the size of digested capsules in molecular sizes, which may enhance identification of the various high molecular weight capsules carrying V. cholerae members. The nature of the polysaccharide biosynthetic genes would also be characterized which may also aid identification. Another area of future research interest is the control of biofilm formation which has enhanced the pathogen environmental survival. Various actinobacterial members are being studied to develop an antibiofilm agent to control and eradicate recalcitrant NSAG/NAG-O1/O139 V. cholerae members. Recently, various Vibrio members have shown production of antibiofilm activity bioagent which are exopolysaccharide-A101, QY101 from culture supernatant of some marine Vibrio cholerae members. The survival and recalcitrancy observed amongst the Vibrio members in the environment and Coastal water bodies would also have been reduced with the advent of antibiofilm biomolecule. There is currently an ongoing study to produced antibiofilm agent from the actinobacterial diverse nature. The future presents possible eradication and control strategy for the pathogen as interest is engendered toward the study of the NSAG/NAG-O1/O139 V. cholerae members.

The clinical relevance of NSAG/NAG-O1/O139 V. cholerae members has remained unclear since most of its members are neglected in the field and/or research driven interest. Standard microbiological, molecular and serological methods for detecting these potential outbreak causing pathogens in the environment are also limited. A possible future direction may be a redirected attention as well as research driven interest on these members and their respective pathogenic potential using effective molecular biology, microbiological protocols and Molecular typing methods. These methods should also employ a well-structured novel technology as an environmental monitoring strategy toward enhancing the detection of the pathogen since they are residential floral of the estuaries and coastal region. A novel technique which may be use for pathogen enumeration, serotyping using the various surface sugar and aminoglycosides to differentiate the members and application of "DNA chip" that will structurally bind to both mobile DNA as well as environmental bacterial of the group be employed. In addition to this, countries and specific health organizations in endemic and pandemic regions of cholera should encourage reporting cases of O1/O139-NAGVc members in any observed region. An awareness campaign and peer educator program must be initiated with a view to eliminating related Vibrio pathogens. The application of these relevant advance methods may also provide result to the detection of Viable but Non-culturable strains (VBNC) of the Vibrio members which are posing threat to the environment. It will also describe a model for the resuscitation, enumeration and detection of the NSAG/ NAG-O1/O139 Vibrio members in aquatic environment. The poor understanding and dynamics for the serological detection of non-O1/non-O139 Vibrio cholerae and the standard method for detecting NSAG/NAG-O1/O139 members has presented this emerging pathogenic group as public health risk associated. A risk situation such that, if not properly handle as early as possible would result a world outbreak situation of cholera. Although the point of discuss that NSAG/NAG-O1/O139 members may play an incidental role in re-establishing epidemic V. cholerae O1 strain has not been justified, it is envisaged that future position of the potential pathogen is not far from such. We believe that a more intense research driven studies be conducted on the emerging pathogen. This strategic intervention study would specifically focus on the environmental resident ethiologic agent known as NSAG/NAG-O1/O139 V. cholerae members. A special interest should be directed at those members with the choleragen (ie the ctx-gene, tcp-gene, cep-gene, ace-gene etc.) and the epidemic associated virulence genes. These are some of our ongoing research, interest and study in our laboratory. The clonal association of these NSAG/ NAG-O1/O139 members in the V. cholerae study is another study area which we are exploring with a view to understanding the dynamism and relationship of the V. cholerae strains. Understanding these will enhance current surveillance of the emerging pathogen to provide the adequate management of infection cases.

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Fluorescent amplified fragment length polymorphism and repetitive extragenic palindrome-PCR fingerprinting reveal host-specific genetic diversity of Vibrio halioticoli-like strains isolated from the gut of Japanese abalone

Genetic and phenotypic analysis of Vibrio cholerae non-O1, non-O139 isolated from German and Austrian patients

Phenotypic and genetic analyses of 111 clinical and environmental O1, O139, and non-O1/O139 Vibrio cholerae strains from different geographical areas

Fish as reservoirs and vectors of Vibrio cholerae

Comparative proteomics and secretomics revealed virulence, and coresistance-related factors in non O1/O139 Vibrio cholerae recovered from 16 species of consumable aquatic animals

Molecular analysis of non-O1, non-O139 Vibrio cholerae associated with an unusual upsurge in the incidence of cholera-like disease in Calcutta, India

Distribution of some virulence related-properties of Vibrio alginolyticus strains isolated from Mediterranean seawater (Bay of Khenis, Tunisia): investigation of eight Vibrio cholerae virulence genes

Characterization of Vibrio cholerae O1 El Tor biotype variant clinical isolates from Bangladesh and Haiti, including a molecular genetic analysis of virulence genes

Brightred'syndrome in Pacific white shrimp Litopenaeus vannamei is caused by Vibrio harveyi

Phylogeny of Vibrio cholerae based on recA sequence

Genetic rearrangements in the rfb regions of Vibrio cholerae O1 and O139

Isolation of human pathogenic bacteria in two edible fishes, Priacanthus hamrur and Megalaspis cordyla at Royapuram waters of Chennai

BOX-PCR is an adequate tool for typing Aeromonas spp

Virulence of cholera toxin gene-positive Vibrio cholerae non-O1/non-O139 strains isolated from environmental water in Kolkata India

Identification of Vibrio isolates by a multiplex PCR assay and rpoB sequence determination

Design and validation of a novel multiplex real-time PCR assay for Vibrio pathogen detection

Faecal pollution loads in the wastewater effluents and receiving water bodies: a potential threat to the health of Sedibeng and Soshanguve communities, South Africa

Notes on the characterization of prokaryote strains for taxonomic purposes

Severe diarrhea caused by cholera toxin-producing vibrio cholerae serogroup O75 infections acquired in the southeastern United States

Evaluation of the microbiological safety and quality of Vietnamese Pangasius hypophthalmus during processing by a microbial assessment scheme in combination with a self-assessment questionnaire

Non-O1, non-O139 Vibrio cholerae bacteraemia in an Australian population

Identification of bacterial repPCR genomic fingerprints using a backpropagation neural network

Comparison of virulence gene profiles and genomic fingerprints of Vibrio cholerae O1 and non-O1/non-O139 isolates from diarrheal patients in southern Thailand

16S rDNA genotyping using PCR/RFLP (restriction fragment length polymorphism) analysis among the family Vibrionaceae

Distribution of repetitive DNA sequences in eubacteria and application to finerpriting of bacterial enomes

An intricate network of regulators controls biofilm formation and colonization by Vibrio fischeri

How Vibrio cholerae survive during starvation

Development and application of real-time polymerase chain reaction to detect Vibrio cholerae O1 and O139 in river water

Detection of Vibrio cholerae O1 and O139 in environmental water samples by an immunofluorescent-aggregation assay

Inhibition of adhesion of intestinal pathogens (Escherichia coli, Vibrio cholerae, Campylobacter jejuni, and Salmonella Typhimurium) by common oligosaccharides

One health pathogen surveillance demonstrated the dissemination of gut pathogens within the two coastal regions associated with intensive farming

Use of REP-and ERIC-PCR to reveal genetic heterogeneity of Vibrio cholerae from edible ice in Jakarta

The characterization of pathogenic microorganisms by genomic fingerprinting using arbitrarily primed polymerase chain reaction (AP-PCR). In: Persing DH (ed) Diagnostic molecular microbiology

DNA polymorphisms amplified by arbitrary primers are useful as genetic markers

Induction of viable but nonculturable state in Vibrio parahaemolyticus and its susceptibility to environmental stresses

Cholera, number of cases. Global health observatory data repository

Deployments from the oral cholera vaccine stockpile

Taxonomic and functional metagenomic profiling of gastrointestinal tract microbiome of the farmed adult turbot

District prediction of cholera risk in China based on environmental factors

Detection and confirmation of toxigenic Vibrio cholerae O1 in environmental and clinical samples by a direct cell multiplex PCR

Distribution of serogroups of Vibrio cholerae non-O1 non-O139 with specific reference to their ability to produce cholera toxin, and addition of novel serogroups

Distribution of Vibrio cholerae O1 antigen biosynthesis genes among O139 and other non-O1 serogroups of Vibrio cholerae

Development of an immunochromatographic test strip for detection of cholera toxin

PCR optimization of BOX-A1R PCR for microbial source tracking of Escherichia coli in waterways

Vibrio biofilms: so much the same yet so different

Enzymatic electrochemical detection of epidemic-causing Vibrio cholerae with a disposable oligonucleotide-modified screen-printed bisensor coupled to a dry-reagent-based nucleic acid amplification assay

Non-O1, non-O139 V. cholerae septicemia at a tertiary care center

A case report and review

We are grateful to the South African Medical Research Council (SAMRC) and Govan Mbeki Research and Development Centre (GMRDC) of Fort Hare University for their financial support. We equally appreciate Prof Nwodo Uchechukwu U. and Prof Okoh Anthony Ifeanyi for the time to read through the manuscript, advice, attention and design given while writing this review.