https://doi.org/10.52973/rcfcv-e34485

Received: 09/07/2024 Accepted: 25/09/2024 Published: 10/12/2024

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Revista Científica, FCV-LUZ / Vol. XXXIV, rcfcv-e34485

ABSTRACT

Sheep production in Mexico encounters notable challenges, among

which infectious diseases stand out as a growing concern. Ovine

respiratory syndrome (ORS) is particularly problematic, being a

leading cause of economic losses in the industry. However, despite

its signicant negative impact, there remains a lack of comprehensive

understanding regarding the microorganisms involved. For this

reason, the aim of this study was to isolate and identify the causal

agents responsible for a respiratory disease outbreak in a sheep

production unit in Northern Veracruz. This included: collection of

samples from affected sheep, focusing on those displaying clinical

signs of respiratory illness; microbial culturing and molecular

identication of the isolated bacteria. We isolated rounded, raised

colonies with a pink mucoid aspect which were molecularly identied

as Enterobacter hormaechei, which exhibited a similarity of 99.59%

with sequences from China. The isolation and molecular identication

of E. hormaechei provide new insights into the pathogens affecting

sheep, highlighting the importance of continuous surveillance and

research in improving sheep health and production. This study

represents a signicant step in identifying and understanding the

causal agents of ORS in Northern Veracruz.

Key words: Enterobacteria; emerging pathogen; respiratory

complex; small ruminant; Mexico

RESUMEN

La producción ovina en México enfrenta desafíos notables, entre los

que destacan las enfermedades infecciosas como una preocupación

creciente. El síndrome respiratorio ovino (SRO) es particularmente

problemático y es una de las principales causas de pérdidas

económicas en la industria. Sin embargo, a pesar de su importante

impacto negativo, sigue existiendo una falta de comprensión

integral sobre los microorganismos involucrados. Por esta razón, el

objetivo de este estudio fue aislar e identicar los agentes causales

responsables de un brote de enfermedad respiratoria en una unidad de

producción ovina del Norte de Veracruz. Esto incluyó: recolección de

muestras de ovejas afectadas, centrándose en aquellas que presentan

signos clínicos de enfermedad respiratoria; cultivo microbiano e

identicación molecular de las bacterias aisladas. Aislamos colonias

redondeadas, elevadas, de aspecto mucoide rosado, que fueron

identificadas molecularmente como Enterobacter hormaechei,

las cuales exhibieron una similitud del 99,59% con secuencias

detectadas en China. El aislamiento y la identicación molecular

de E. hormaechei proporcionan nuevos conocimientos sobre los

patógenos que afectan a las ovejas, destacando la importancia de

la vigilancia y la investigación continuas para mejorar la salud y la

producción de las ovejas. Este estudio representa un paso importante

en la identicación y comprensión de los agentes causales de la SRO

en el norte de Veracruz.

Palabras clave: Enterobacteria; patógeno emergente; complejo

respiratorio; pequeños rumiantes; México

First isolation and molecular identication of Enterobacter hormaechei in a sheep

production unit with respiratory syndrome from Northern Veracruz, Mexico

Primer aislamiento e identicación molecular de Enterobacter hormaechei en una unidad de

producción de ovinos con presencia de síndrome respiratorio en el Norte de Veracruz, México

Javier Cruz Huerta–Peña

, Gabriela Romina Hernández–Carbajal

, Gerardo Gabriel Ballados–González

José Manuel Martínez–Hernández

, José Alfredo Villagómez–Cortés

, Sokani Sanchez–Montes

Universidad Veracruzana, Facultad de Ciencias Biológicas y Agropecuarias, región Poza Rica Tuxpan. Veracruz, Mexico.

Universidad Veracruzana, Facultad de Medicina Veterinaria y Zootecnia, Veracruz, Mexico.

*Corresponding author: sok10108@gmail.com

Isolation and molecular identification of Enterobacter hormaechei in sheep / Huerta–Peña et al. ___________________________________

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INTRODUCTION

Sheep (Ovis aries) production in Mexico represents one of the

four most important sectors in the generation of animal protein

for national consumption. It is estimated that there are 5,714,882

sheep nationwide. In fact, Veracruz state is one of the top 10 states

in terms of sheep population, accounting for 4.40% of the national

production, with 251,322 animals in production units [1]. Particularly,

the North of Veracruz concentrates 25% of the state’s production,

which 62,903 animals.

Sheep national production indeed faces signicant challenges,

with infectious diseases emerging as a growing problem [2, 3]. Ovine

respiratory syndrome (ORS) represents one of the main causes of

economic losses because it affects 10% to 40% of sheep, being a

leading cause of death [4]. In lambs, this syndrome led to signicant

adverse effects such as mortality and poor quality of lambs produced

[4, 5]. The ORS is caused by a complex interaction of factors,

including the presence of opportunistic bacteria (key pathogens

involved include Mannheimia haemolytica, Bibersteinia trehalosi,

Pasteurella multocida, Mycoplasma spp., and Escherichia coli, which

are typically harmless but can invade the respiratory tract under

certain conditions, leading to disease), environmental conditions

(particularly, extreme temperature changes and poor ventilation),

and inadequate animal husbandry practices (such as overcrowding,

weaning time, transport to other facilities, mixing animals from

different origins, and coexistence of generational strata) [2, 3, 4, 5, 6].

In the state of Veracruz, there is a lack of information related to

the surveillance and molecular typing of microorganisms causing

ORS in sheep ocks. For this reason, the aim of the present study

was to identify the causal agents of an outbreak of ORS in a sheep

production unit in Northern Veracruz, Mexico. By isolating and

molecularly characterizing the pathogens involved, this research

aims to contribute to a better understanding of the epidemiology and

management of respiratory diseases in sheep populations.

MATERIAL AND METHODS

Sampling

The study was conducted in a sheep production unit located in the

municipality of Tihuatlan, Veracruz, within the Huasteca Baja region

of Northern Veracruz. The municipality’s geographical coordinates

are 20°43'1" N, 97°32'13" W, and it is situated at an altitude of 105

MASL. Median temperature is 30.7°C, relative humidity about 63–65%,

and precipitation of 15.8–16.0 mm. The production unit comprises

approximately 500 hair sheep.

Study population

In May 2022, lambs and adult animals in the production unit

exhibited respiratory signs such as expectoration, rhinorrhoea,

lethargy, and loss of appetite. These symptoms were accompanied by

an alarming increase in mortality rates among the sheep. In response

to the situation, animals showing signs of illness were quarantined,

and further investigation was initiated to identify potential causal

agents. A total of 30 sheep were sampled, 22 were females and

8 males, with ages ranging from one month to two years, with an

average of 1.5 years.

During the investigation, sheep were physically restrained, and

demographic data along with physiological constants (temperature,

respiratory rate and heart rate) of each animal were recorded. After

physical restraint, the exterior of the nose of each animal was

disinfected with Mycrodacyn, and a sterile Dacron®/polyester swab

was inserted into the nostril and rotated against the wall of the nasal

cavity. Nasal swab samples were collected from the affected animals

and preserved in 15 mL conical tubes containing sterile saline to

conserve bacterial and mycotic agents. Subsequently, the samples

were maintained in a cold chain to preserve their integrity until their

arrival at the laboratory for analysis.

Bacterial and mycotic isolation

Samples taken individually streaking nasal swab were inoculated

directly onto selective agar media (MacConkey and blood agar for

bacterial isolation, and Sabouraud Dextrose Agar, Emmons with

Gentamicin for fungal isolation) which were incubated (Ecoshel,

91210, Pharr, USA) at 37°C for 72 hours (h) and checked every 12 h for

the presence of microbial growth.

Molecular identication of bacterial isolates

On each solid culture plate with growth, several colonies of interest

(with similar morphology, size and coloration) were selected for DNA

extraction. They were placed with the help of a microbiological loop

in 1.5 mL low–adherence conical tubes (LoBbind). For each tube

we added 500 µL of a 10% Chelex 100 chelating resin solution (Bio–

Rad®, United States of America (USA) with 20 µL of proteinase K

(SIGMA life sciences®, USA) and incubated at 56°C for one hour (IVYX

Scientic, 0745556232573, Washington, USA). Subsequently, the

temperature was increased to 94°C for 15 min to denature excess

of proteins and were centrifuged at 8,000 G (Hsiang Tai Model

CN–3600, Taiwan, China) for 15 min. Samples were allowed to cool

to room temperature, supernatant were recovered in new tubes and

then frozen at -20°C until use (Hisense®, FC88D6BWX1, China). A

450 bp fragment of the 16S ribosomal gene was amplied in a Veriti

96–Well Fast Thermal Cycler (ThermoFisher Scientic, 4375305,

Massachusetts,USA). The reaction mix consisted of 12.5 µL of GoTaq®

Green Master Mix, 2× Promega Corporation (Madison, WI, USA), 1µL

of each oligonucleotide (EHR01 GCCTAACACATGCAAGTCGAACG

and EHR02 GCCCAATAATTCCGAACAACG) [7], 1 µL of DNA (50 ng)

and 9.5 µL of nuclease–free water. We followed the thermal PCR

conditions previously proposed [7]. PCR products were visualized

by electrophoresis (Shelton Scientic®, QS–710, EUA) in 2% agarose

gels stained with Midori green and run with 1% TAE running buffer

solution at 85V for 40 min. Positive amplicons were sent for

sequencing (Applied BiosystemsTM, 3130xl, EUA) to Macrogen, Korea.

The sequences obtained in this study were aligned with those of

other validated bacterial species from the same genera deposited

in GenBank using the Clustal W algorithm in MEGA 10. We selected

the nucleotide substitution model based on the lowest AICc (Akaike

information criterion, corrected). A phylogenetic reconstruction was

generated using Maximum Likelihood, with 1000 Bootstrap replicates,

using the close neighbour interchange method. Gaps were excluded

from the analysis.

RESULTS AND DISCUSSION

The physiological constants recorded in the 30 sampled animals

were as follows: Temperature 39.84 ± 0.75 (39–41) °C, respiratory

rate 17.84 ± 2.95 (14–24) BPM, and heart rate 82.68 ± 9.38 (70–97)

BPM. A total of 22 positive culture media for bacterial growth were

FIGURE 1. Maximum likelihood phylogenetic tree generated using T93 + G+I

distance model with partial sequences of the 16S rRNA gene from several members

of the genus Enterobacter. Bootstrap values greater than 50 are indicated at the

nodes. Sequences generated in this study are marked with solid forms

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obtained, which described rounded, raised colonies with a pink

mucoid aspect. None of the Sabouraud media were positive for

fungal growth. All media with growth were tested for the detection

of bacterial using universal 16S rDNA primers. Males exhibited the

highest percentage of infection with an 87.5% (7/8), followed by

females with 68.18% (15/22), representing a frequence of 73.33%

(22/30). However, we only recovered 20 sequences with adequate

quality for phylogenetic analysis.

The set of 20 consensus sequences obtained had 490 bp, coverage

of 99–100%, and similarities ranging 99.59% with sequences of

Enterobacter hormaechei from China (GenBank Accession numbers

MN007139.1 and KJ660958.1). Sequences generated in this study

were deposited in GenBank under the following accession numbers:

PP893165–PP893184. The ML reconstruction grouped our sequences

in the same branch with other E. hormaechei sequences deposited

in GenBank supported by a bootstrap value of 63%. (FIG. 1).

Ovine respiratory syndrome is commonly attributed to bacterial

agents of the Pasteurella, Mannheimia, Bibersteinia, and Mycoplasma

genera, the inclusion of E. hormaechei among the bacterial agents

is notable [2, 4, 5, 6].

The identification of E. hormaechei in sheep with respiratory

problems marks a signicant discovery, particularly as it is the rst

report of this microorganism in ORS in Mexico and Latin America.

This suggests a potential emerging pathogen in sheep populations

in the region. E. hormaechei is a Gram–negative oxidase–negative,

fermentative bacterium and a member of the Enterobacter cloacae

complex (ECC), is primarily known for its significance in human

clinical settings, where it can cause serious nosocomial infections

[8]. Its presence in ORS adds a new dimension to our understanding

of respiratory diseases in ovine populations [4, 8]. The identication

of E. hormaechei expands this list and underscores the importance

of considering a broad range of potential pathogens in the diagnosis

and management of respiratory diseases in sheep.

This discovery highlights the need for further research into the

prevalence, transmission dynamics, and impact of E. hormaechei

on sheep health and production in Mexico and Latin America.

Understanding the role of this microorganism in ovine respiratory

diseases can inform preventive measures and treatment strategies

to better protect sheep populations and enhance overall herd health.

The expanding recognition of E. hormaechei as a potential pathogen

in various animal species accentuates its importance in veterinary

medicine and highlights the need for increased awareness and

surveillance of this microorganism. Reports of E. hormaechei in

different animal species, including pigs, foxes, and cattle, suggest

its ability to infect a wide range of hosts and potentially cause

various clinical conditions, from diarrhoea in piglets to severe

respiratory conditions in calves [9, 10, 11]. The recent identication

of E.hormaechei as the causative agent of fatal respiratory conditions

in calves and lambs in China emphasizes the significance of

understanding its role in animal health and disease [8, 9, 10].

Recently, the isolation of E. hormaechei from lung tissue samples of

sheep, as well as its genetic similarity to strains from cattle, suggests

a possible cross–species transmission route which is strengthened

by the ndings of the present study [8, 9, 10]. In the context of the

farm studied in the present study, where dual–purpose cattle are

present, but no effective preventive medicine program is in place,

the lack of biosecurity measures such as sanitary mats or controlled

movement between cattle grazing sites and sheep sheds may

facilitate transmission, potentially through fomites. The observation

of a high number of animals per square meter, experiencing rapidly

evolving respiratory problems leading to increased mortality suggests

a signicant health challenge within the sheep population on the

analysed farm. Several factors may contribute to this situation, like

immunosuppression triggered by seasonal changes and decreasing

temperatures [4, 5, 6]. Respiratory diseases in sheep are often

exacerbated during periods of environmental stress, such as seasonal

transitions, which can weaken the animals’ immune system and

increase their susceptibility to infections [4, 6].

Multiple reports of resistance to a wide range of antibiotic therapies

by this species of Enterobacter exist [11, 12, 13], particularly to β–

lactam and quinolone, which are widely used in the human clinic,

which is why this species must be approached from the perspective

of comprehensive perspective of One Health to reduce the risk of

circulation between species and establishment in humans [10, 12, 13].

Despite regular treatment with enrooxacin in animals from the

studied farm, the persistence of respiratory problems suggests a

potential issue with treatment ecacy. The literature indicates that

resistance to quinolones, including enrooxacin, is a growing concern

in veterinary medicine, with many strains of bacteria exhibiting

resistance to these antibiotics [12, 13].

Isolation and molecular identification of Enterobacter hormaechei in sheep / Huerta–Peña et al. ___________________________________

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In this study, the lack of establishment of an antibiotic susceptibility

profile for the recovered colonies hinders the ability to identify

potential antibiotic resistance. Understanding the susceptibility

of bacterial isolates to antibiotics is crucial for guiding appropriate

treatment strategies and preventing the spread of resistant strains.

Moving forward, it is essential to conduct a comprehensive

antibiotic susceptibility testing on bacterial isolates from affected

animals to determine the most effective treatment options.

Additionally, apply strategies to minimize the risk of antibiotic

resistance, such as prudent antibiotic use, surveillance of resistance

patterns, and implementation of infection control practices, is crucial

for maintaining animal health and welfare on the farm.

CONCLUSIONS

In this work, the presence of E. hormaechei with a frequence

of 73.33% was detected for the rst time through microbiological

isolation and molecular typing in sheep with respiratory symptoms

in a livestock farm in the North of Veracruz, which suggests that

these bacteria must be monitored as a possible causal agent of ORS

in Mexico and other Latin American countries. Continued research is

essential to explore the prevalence, impact, and control strategies

for E. hormaechei and other pathogens in sheep populations.

ACKNOWLEDGMENTS

We thank the local producers for their collaboration to get this

study completed. We are grateful to the undergraduate students

of the Veterinary Medicine program for their support to accomplish

this study.

Declaration of competing interest

The authors declare that they have no known competing nancial

interests or personal relationships that could have appeared to

inuence the work reported in this paper.

Funding

Not applicable.

Ethical approval

The authors conrm that the ethical policies of the journal, as noted

on the journal’s author guidelines page, have been adhered to. This

study was approved by the Bioethics Committee of the Facultad de

Ciencias Biológicas y Agropecuarias, Campus Poza Rica–Tuxpan of

the Universidad Veracruzana (UV) (Animals were handled according

to National Legislation and Ethics (NOM–012–ZOO–1993).

Data availability

All datasets used and/or analyzed during this study are included in

this article. Sequences generated are deposited in GenBank under

Accession numbers: PP893165–PP893184.

Consent to participate

Not applicable

Consent for publication

Not applicable

Author contributions

Javier C. Huerta–Peña: Conceptualization, Data curation, Investigation,

Methodology, Writing – original draft. Gabriela R. Hernández–Carbajal:

Conceptualization, Data curation, Investigation, Methodology, Writing –

original draft. Gerardo G. Ballados–González: Investigation, Supervision,

Writing – original draft, Writing – review and editing. José M. Martínez–

Hernández: Investigation, Supervision, Writing – original draft, Writing –

review and editing. José A. Villagómez–Cortés: Investigation, Supervision,

Writing – original draft, Writing – review and editing. Sokani Sánchez–

Montes: Conceptualization, Data curation, Formal analysis, Funding

acquisition, Investigation, Project administration, Writing – original

draft, and Writing – review and editing.

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