Scholarly article on topic 'Effect of Henna (Lawsonia inermis) extract on the immunity and survival of common carp, Cyprinus carpio infected with Aeromonas hydrophila'

Effect of Henna (Lawsonia inermis) extract on the immunity and survival of common carp, Cyprinus carpio infected with Aeromonas hydrophila Academic research paper on "Veterinary science"

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Int Aquat Res
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Academic research paper on topic "Effect of Henna (Lawsonia inermis) extract on the immunity and survival of common carp, Cyprinus carpio infected with Aeromonas hydrophila"

Int Aquat Res (2016) 8:247-261 DOI 10.1007/s40071-016-0141-2



Effect of Henna (Lawsonia inermis) extract

on the immunity and survival of common carp, Cyprinus

carpio infected with Aeromonas hydrophila

Siyavash Soltanian . Mohammad Saeid Fereidouni

Received: 30 December 2015/Accepted: 3 August 2016/Published online: 16 August 2016 © The Author(s) 2016. This article is published with open access at

Abstract In this study, the immunomodulatory properties of Lawsonia inermis (henna) in common carp, Cyprinus carpio was investigated. Fish were intraperitoneally (i.p.) injected with 6, 60 or 600 mg kg- body weight (BW), of the methanolic soluble fractions of L. inermis. The extract at 60 and 600 mg kg-1 BW, significantly (p < 0.05) enhanced some non-specific immune parameters such as serum lysozyme and bactericidal activity, phagocytic and respiratory burst activity, total leucocyte count (TLC), lymphocyte, monocyte and neutrophil number. Disease resistance against Aeromonas hydrophila has also been improved following herbal treatment. This preliminary study indicates the beneficial effect of L. inermis in improving immune status and controlling infectious diseases in aquaculture.

Keywords Lawsonia inermis • Common carp • Immune response • Aeromonas hydrophila • Disease resistance


Chemotherapies are widely used by farmers to control and prevent diseases, which have several drawbacks such as environmental risks, development of resistant pathogens and bioaccumulation (Rao et al. 2006). Nowadays, several alternative strategies such as immunostimulants, probiotics, green water technique, vaccination and quorum sensing have been introduced in aquaculture to improve fish resistance to pathogen and improve growth performance (Markestad and Grave 1997; Brekke 1998; Sakai 1999; Rodgers and Furones 2009; Defoirdt et al. 2011; Romero et al. 2012; Sihag and Sharma 2012; Revertera et al. 2014).

Mello et al. (2013) observed an increase in intestinal goblet cell count (GC) in tilapia fed dietary probiotic supplementation. The increase in GC may enable an increase production of mucous, thus increasing intestinal protection against bacterial pathogen.

Immunostimulants mainly facilitate the function of phagocytic and natural killer cells, complement, lysozyme and antibody responses of fish. These effects depends on various factors like timing, dosage and method of administration as well as the physiological condition of the fish (Harikrishnan et al. 2011).

Various kinds of substances have been used and their suitability as immunostimulant has been studied, but only few of them are found suitable for use in aquaculture (Raa et al. 1992; Siwicki et al. 1998). Recently,

S. Soltanian (&) • M. S. Fereidouni

Aquatic Animal Health and Diseases Department, School of Veterinary Medicine, Shiraz University, 71441-69155 Shiraz, Iran

e-mail: M. S. Fereidouni


growing interest has been paid to herbal based immunostimulants in aquaculture. Herbal products are cheaper source for therapeutics and biocompatible, biodegradable and safe for the environment (Ortuno et al. 2002; Bricknell and Dalmo 2005).

Lawsonia inermis Linn, popularly known as henna plant, belongs to the family of Lythraceae.

The henna plant is native to North Africa and South-West Asia. It is cultivated in Kerman, Hormozgan, and Baloochestan province of Iran (Rechinger 1968). Henna leaves are very popular natural dye to color hand, finger, nails and hair (Joshi 2000). It contains a pigment called Lawson (2-hydroxy-1, 4-naphthoquinone), mannitol, mucilage, flavonoids such as apigenin, luteolin, quercetin, several phenolic glycosides, coumarin, xanthone, quinoids, glycosides, beta-cytostrol, terpenoids, lipid, resin, tannin, catechin and essence. Other compounds derived from henna leaves are 5-7 glycosides derivatives, gallic acid, acastin glycoside, laxanthon 1 and 2, and small amount of alkaloids (El Babili et al. 2013).

The plant extract or its purified compounds exhibit a variety of biological activities such as antimicrobial activity (Malekzadeh 1968; Abdel-Malek et al. 1973), anti-sickling activity (Chang and Suzuka 1982; Clarke et al. 1986), hepatoprotective activity (Anaad et al. 1992), cytotoxic activity (Ali and Grever 1998), antiinflammatory, antipyretic, and analgesic activities (Ali et al. 1995). Furthermore, anti-diarrheal, antioxidant and regenerative properties as well as neutralizing the free radicals have been reported (Prakash et al. 2007). Moreover, L. inermis has also been used in ethno-medicine to treat various maladies including arthritis, headaches, ulcers, diarrhea, leprosy, intestinal neo-plasticity, jaundice, fever, leucorrhoea, diabetes, and small pox (Elmanama et al. 2011). In addition, in vitro immunomodulatory properties of henna leaves have also been reported (Dikshit et al. 2000; Mikhaeil et al. 2004). More recently, the methanolic extract of L. inermis has been shown to exert an immunomadilatory effect in striped murrels (Channa striatus) (Uthayakumar et al. 2014a). Therefore, the aim of this study was to determine the immunomadilatory activity of L. inermis methanolic extract in common carp.

Materials and methods

Experimental fish

Apparently healthy juvenile common carps, with an average initial weight of 46.25 ± 8 g were obtained from a fish farm in Shiraz, Fars province, south west of Iran. Fish were acclimated to laboratory conditions in glass tanks for a period of 2 weeks. The health status was examined microbiologically throughout the acclimatization period. During the experimental period, the water was measured at 25 ± 2 °C, dissolved oxygen 5-5.5 ppm and pH 7-8. Ammonia, nitrite and nitrate were monitored using a commercial testing kit (Fish Farming Test Kit, Model FF-1A; HACH Co., Loveland, CO, USA) and maintained in standard ranges. During the acclimation and sampling periods, fish were fed twice daily a commercial carp pelleted food (Table 1, Beyza Technology Co., Ltd., Iran) at a feeding rate of 3 % body weight.

Table 1 Composition of commercial diet

Nutrients Value

Gross energy (Kcal/Kg) 3500

Crude protein (%) 35-37

Crude lipid (%) 9-11

Crude fiber (%) 5 %

Moisture (%) <10

Ash (%) <10

TVN (mg/100 g) <45

TVN total volatile nitrogen Springer

Herbal extract

Lawsonia inermis medicinal plant was collected from herbal medicine shop and its identity was confirmed using monographs by Mozaffarian (1996). About 150 g of powdered leaves was taken in a clean, flat bottomed glass container and soaked in 1.5 L of 85 % methanol. The container with its contents was sealed and kept for a period of 7 days accompanying occasional shaking and stirring. The whole mixture then underwent a coarse filtration by a piece of clean, white cotton material. Then, it was filtered through Whatman filter paper (Bibby RE200, Sterilin Ltd., UK). The obtained filtrate (methanol extract) was evaporated using a rotary evaporator. It rendered a gummy concentrate of reddish black color. The gummy concentrate was designated as a crude methanol extract of methanol. The extract was stored in a refrigerator (4 °C) until used.

Experimental design

The experimental fish were divided randomly into four groups (ninety-two fish/group in four replicates) for administration of different doses of methanolic extract of L. inermis injected intraperitoneally (200 iL) with the following preparations: T1 control (injected with PBS), T2, injected with 6 mg kg-1 methalonic L. inermis extract, T3, injected with 60 mg kg-1 methalonic L. inermis extract, T4, injected with 600 mg kg-1 methalonic L. inermis extract. Before injection, the extract was filter-sterilized using 0.2 im membrane filters (Whatman, UK).

Blood and serum collection

The fish were bled 2 days prior to and 2, 4, 6, 8 and 10 days after treatment. Six fish from each group were randomly selected and anesthetized using MS 222 (0.1 ppm). The blood samples were collected from caudal vein using a 2-mL syringe and a 24-gauge needle.

Sampled fish were not returned to the experimental population and were euthanized using an over dose (300 ppm) of MS 222. One part of each blood sample was transferred into preheparinised plastic Eppendorf tubes while the other part was transferred into tubes or Eppendorf tubes without anticoagulant and was allowed to clot for 2 h at room temperature in a slanting position. Before the serum was collected, the tubes were kept at 4 °C overnight and were then centrifuged at 2500xg for 15 min. The serum was stored at -20 °C in screwcap glass vials until use.

Determination of serum biochemical and hematological parameters

Blood samples were immediately analyzed for the estimation of numbers of erythrocytes (RBC) and leucocytes (WBC), Hemoglobin (Hb) and Hematocrit levels (% red blood cells). RBC and WBC counts were performed as described by Schaperclaus et al. (1991). Hemoglobin contents (Hb) were determined using cyanmethemoglobin method with Drabkin's solution (Goldenfarb et al. 1971). Hematocrit was determined by the microhematocrit method (Fox et al. 1997). The leukocyte differential count was done in peripheral blood smears stained with May-Grunwald/Giemsa stains. Leucogram was assessed for each fish under an oil immersion lens. One hundred white blood cells from each smear were assessed and the percentage of different types of leucocytes was calculated (Schaperclaus et al. 1991).

Total serum protein was measured by the Biuret method (Kwapinski 1965). Total serum immunoglobulin (Ig) was measured as previously described by (Siwicki and Anderson 1993). First, Ig was separated from serum by precipitation with polyethylene glycol and remaining protein in the supernatant was assayed. That amount was subtracted from the total protein to give total Ig.

Phagocytic assay

Phagocytic activity was measured following (Siwicki and Anderson 1993) with slight modifications. The heparinized blood was immediately used for the phagocytic assay. Briefly, 1 x 107 cells of Staphylococcus aureus in 0.1 mL of PBS were added to 0.1 mL of blood samples in a microplate. This was then incubated for 30 min at 25 °C after thorough mixing in the well.

After incubation, the plate was mixed gently, and 0.05 mL of this suspension was smeared on the glass slide. After air drying, the smears were fixed in ethanol and stained with Giemsa (7 %). The phagocytic cells were counted. Phagocytic activation (PA) was determined by enumerating 100 phagocytes per slide under a microscope. The mean of the slides was calculated as below; PA: (Number of phagocytic cells with engulfed bacteria/number of phagocytes) x 100.

Lysozyme assay

Serum lysozyme activity was determined using the methods described by (Jian and Wu 2003). Briefly, a suspension of an overnight grown Micrococcus lysodeikticus was prepared by dissolving 20 mg of M. lysodeikticus into 100 mL of 0.067 mol/L PBS (pH 6.4) and then, 100 iL of fish serum was added to a 3 mL suspension of M. lysodeikticus. The reaction was carried out at 25 ± 1 °C, and an absorbance at 540 nm was measured after 0.5 and 4.5 min. One unit of lysozyme activity was defined as the amount of lysozyme producing a decrease in absorbance of 0.001/min.

Respiratory burst activity

Oxidative radical production by neutrophils during respiratory burst was measured by the NBT assay as described by (Anderson and Siwicki 1995). Briefly, blood and 0.2 % NBT were mixed in equal proportion (1:1), incubated for 30 min at 25 °C, and then 50 iL was taken out and dispensed in glass tubes. For solubilisation of reduced formazen product, 1 mL of dimethylformamide (Sigma, USA) was added and centrifuged at 2000xg for 5 min. Finally, the supernatant was taken and the extent of NBT reduced was measured at an optical density of 540 nm. Dimethyl formamide was used as the blank.


A virulent strain of Aeromonas hydrophila (Dehghani et al. 2012), was obtained from Aquatic Animal Health and Diseases Department, Shiraz University, Iran. The virulent strain was isolated from infected fish originating in Iran (Modarres Mousavi Behbahani et al. 2014). Stock cultures were maintained at -70 °C in a suspension of tryptic soy broth (TSB) containing 15 % glycerol. For the preparation of bacteria for challenge test, A. hydrophila from stock was cultured for 24 h at 25 °C in TSB. The cells were centrifuged (3000xg for 15 min) and washed three times with sterile (PBS, pH 7.2). The bacterial suspension was adjusted to an optical density of 0.5 at 540 nm, which had been determined to correspond to approximately 10 CFU ml- . After use, the CFU of the bacterial suspension was counted by the spread plate method on tryptic soy agar (TSA) plates.

Challenge experiment

After the administration of plant extracts, 18 fish from the forth replicate in each group were intraperitoneally injected with 0.1 mL of a 24 h growth of virulent A. hydrophila (1 x 108 cells/fish) on day 7. Previously, the challenge dose was adjusted to give 50 % mortality (LD50) in the untreated groups. Mortality was recorded for 15 days. All dead fish and the survivors were examined bacteriologically to determine the presence of the pathogen. The relative percent survival (RPS) was calculated according to Amend (1981):

RPS = [1 - (Mortality (%) in treated group)/(Mortality (%) in control group)] x 100 Serum bactericidal activity

Serum bactericidal activity was determined using the procedure described by Rao et al. (2006). A. hydrophila bacterial culture was centrifuged (3000xg for 15 min) and the pellet was washed and suspended in PBS. OD of the suspension was adjusted to 0.5 at 546 nm. This bacterial suspension was serially diluted (1:10) with PBS five times. Serum bactericidal activity was determined by incubating 2 mL of this diluted A. hydrophila suspension with 20 mL of serum in a micro-vial for 1 h at 25 °C. In the bacterial control group, PBS replaced

the serum. After incubation, the number of viable bacteria was determined by counting the colonies grown on nutrient agar plate for 24 h at 25 °C.

Statistical analysis

Data are presented as Mean ± SD of the number of fish per group. Hematological and immune parameters were analyzed by one way analysis of variance (ANOVA) and Tukey's multiple comparison range. All statistical analyses were tested at the 0.05 level of probability, using the software SPSS 16.0 for Windows.


Phagocytic and NBT activity

Phagocytic activity was significantly enhanced after administration of both medium and high doses of plant extract, peaked on day 8 and 10 (Fig. 1a). NBT activity was significantly higher in groups administered with medium and high doses of plant extract (Fig. 1b). The maximum level was observed in medium dose treatment, recorded on day 10.

Serum lysozyme activity

On most of the days tested, higher serum lysozyme activity was observed in medium and high dose treatment, which was more significant in medium dose treatment (Fig. 1c).

Serum biochemical and hematological parameters

The effects of different levels of henna extract on hematological and biochemical parameters of common carp are shown in Fig. 1a-j; Table 2. The Hb, Hct and RBC values were not affected by all three dosages of plant extract (p > 0.05) (Table 2).

Total serum protein content in the fish injected with either medium dose (60 mg kg-1 BW) or high dose (600 mg kg- BW) of plant extract was significantly (p < 0.05) higher than control fish on day 6, 8 and 10 post- treatment (Fig. 1d), peaked on day 10, in the fish received the medium dose (60 mg kg-1 BW).

Serum globulin content was significantly higher than control on day 8 only in the fish injected with high dose (600 mg kg- BW) of plant extract and on day 10 in the fish treated with both medium and high doses of plant extract (Fig. 1e). However, no significant (p > 0.05) impact on serum globulin level was observed in other groups on different days tested.

After the treatment, an increasing trend was observed in WBC number on all the assay days (Fig. 1f). Both medium and high doses of plant extract could significantly increase the number of WBC on the 6th and 8th day in comparison with control fish.

Fish leucogram was significantly affected by plant extract administration. On all days tested, significantly, lower percentage (proportion) of lymphocytes was observed in fish administrated with both medium and high doses of plant extract compared with the control group (Fig. 1g), although the total number of lymphocyte remained unchanged.

Despite to lymphocytes, the number of monocytes and granulocytes was always significantly enhanced in both medium and high dose treatments in comparison to control group (Fig. 1h, i), yet, a decreasing trend in the number of these cells was observed from day 6 and 8 onwards, respectively.

Serum bactericidal activity

During the assay period, the number of viable bacterial colonies showed a time course dependent decreasing trend in the fish treated with plant extract. Serum bactericidal activity was lowest in the control group and highest in T4 and T5 group recorded on day 10 (p < 0.05) (Fig. 1j). The viable bacterial counts were

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Fig. 1 Hemato-immunological parameters in common carp intraperitoneally injected with single doses of 6, 60 and 600 mg kg-1 BW fish of a methanolic extract of Henna (L. inermis) on days 2, 4, 6, 8 and 10 post-injection. a Phagocytic activity; b NBT activity; c lysozyme activity; d serum total protein level; e serum immunoglobulin level; f WBC number; g lymphocyte (%); h monocyte (%); i granulocyte (%); j serum bactericidal activity. Bars represent mean ± SD from six fish sampled at each time point (n = 6). Different letters over bars represent significant difference (p Tukey < 0.05)

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significantly (p < 0.05) lower in T4 and T5 group compared with either untreated control group or bacterial control (without serum treatment).

Disease resistance

The mortality rate was decreased (Table 3) in fish challenged with virulent A. hydrophila by extract administration. The mortality percentage was found highest (55.5 %) in the control group (infected fish) and lowest (27.7 %) in T5 group. The RPS value was significantly highest (50.0 %) in T5 group followed by T4 and T3 group, respectively (p < 0.05) (Table 3).


In the recent years, there is an increasing interest in the use of herbal extracts for disease control and prevention in aquaculture, indicating that they can modulate immune function in farmed species.

The major components of fish immune system are macrophages, monocytes, granulocytes, and humoral elements, such as lysozymes, immunoglobulins and the complement system (Secombes and Fletcher 1992; Magnadottir 2006). In this study, following i.p. administration of methanolic soluble fractions of L. inermis leaves at different doses (6, 60 and 600 mg kg-1 BW), Several immune parameters such as phagocytic and NBT activities, serum immunoglobulin, lysozyme and total protein level, RBC and WBC number, hematocrit and Hb value, the percentage of lymphocyte (%), monocyte (%), neutrophil (%) and serum bactericidal activity were evaluated in 2 days intervals (Table 2; Fig. 1a-j).

Data showed that methanolic extract of L. inermis significantly enhanced the non-specific humoral and cellular responses and disease resistance against A. hydrophila. All the above immune indices, however, were found to be affected in a time and dose-dependent manner.

Previously, in vitro studies revealed that the methanolic extract of L. inermis displayed immunostimulatory effect as indicated by an enhanced macrophage-stimulating activity and promotion of T-lymphocyte proliferative responses in human (Wagner et al. 1988; Mikhaeil et al. 2004).

Phagocytosis and killing activity by neutrophils and macrophages is an important defense mechanism against pathogenic bacteria (Rao et al. 2006). Previously, enhancement of phagocytic and NBT activities following administration of herbal products in fish species have been reported in a number of studies (Rao et al. 2006; Sahu et al. 2007; Punitha et al. 2008; Pratheepa et al. 2010; Sharma et al. 2010; Behera et al. 2011; Uthayakumar et al. 2014b; Anusha et al. 2014).

In this study, phagocytic activity was significantly enhanced in the common carp after administration of both medium and high doses of plant extract, peaked on day 8 and 10 post- treatment. Similar results were found in Carassius auratus fed crude extracts and purified fractions of Ixora coccinea incorporated in diet (Anusha et al. 2014).

Likewise, NBT activity was significantly higher in groups treated with medium and high doses of plant extract. However, for both phagocytic and NBT activities, maximum values were observed in medium dose treatment recorded on day 10.

Lysozyme plays an important role in innate immunity by lysis of bacterial cell wall and thus stimulates the phagocytosis of bacteria. In this work, the most significant highest lysozyme activity was observed in medium dose treatment. In a similar study, following intraperitoneal administration of different doses (4, 40 or 400 mg kg-1 BW) of water extract of Solanum trilobatum leaves in Oreochromis mossambicus, only the medium dose (40 mg kg- BW) could significantly enhance lysozyme activity on day 4, 6 and 8 post-treatment (Divyagnaneswari et al. 2008). In another study, among various doses of an aqueous extract of Polygonum minus leaf, intraperitoneally injected to African catfish, Clarias gariepinus, only the dose of 15 mg kg-1 BW of plant extract could significantly improve lysozyme activity 2 days post-treatment (Veerasamy et al. 2014). Similar results of elevated lysozyme activity following herbal treatments have been reported (Jian and Wu 2003, 2004; Rao et al. 2006; Yin et al. 2006; Anusha et al. 2014).

Serum protein level is an important indicator of humoral defense system and health status of fish species. In fact, immunostimulants can stimulate protein synthesis to produce more of the molecules involved in immunity such as immunoglobulins, complement, lysozyme, and anti-proteases (Rao et al. 2006). This study revealed that administration of both medium and high dose of henna extract could significantly increase both serum protein and immunoglobulin level in common carp. The increase in serum protein content might be in part due to an increase in the WBC number, which is a major source of serum protein production such as immunoglobulin, lysozyme, complement factors and bactericidal peptides (Misra et al. 2006a, b). This is supported by an enhancement in WBC number in the group that administrated with medium or high dose of henna extract.

A significant increase was reported in serum protein and total immunoglobulin level of rainbow trout fed basal diet incorporated with 1, 2.5 and 5 % black Cumin Seeds, Nigella sativa for 21 days (Dorucu et al. 2009). Furthermore, dietary garlic, onion and ginger could significantly increase total immunoglobulin level in rainbow trout (Nya and Austin 2009) and in the brown marbled grouper, Epinephelus fuscoguttatus (Apines-Amar et al. 2012). In addition, elevated total protein and globulin was reported following administration of medicinal plants in fish species (Dugenci et al. 2003; Misra et al. 2006a; Rao et al. 2006; Yins et al. 2008; Alishahi et al. 2010, 2012; Alishahi and Abdy 2013).

Hematological parameters are used as an index of fish health status to detect physiological changes following different stress conditions such as abnormalities caused by immunostimulants (Agrawal and Mahajan 1980). In this study, no significant difference in the haemoglobin, hematocrit and total erythrocyte count was observed following herbal administration indicating that at such treatment condition no toxic reactions detrimental to the fish were elicited.

Total and differential leucocyte counts are important indices of non-specific defense activities in fish (De Pedro et al. 2005).

Treatment with either medium or high dose of L. inermis extract significantly increased total leukocyte count (TLC) as well as lymphocytes, monocytes and neutrophils number compared with control group. However, maximum effect was observed on day 8 in medium dose treatment. This increment might be in part due to the activation of the haemopoietic tissues by L. inermis as previously reported in rainbow trout following in vitro treatment of macrophages with Glycyrrhiza glabra extract (Jang et al. 1995). Similar

Table 2 RBC, Hct and Hb valuesin common carpintraperitoneally injected with single doses of 6, 60 and 600 mg kg 1 BW fish of a methanolic extract of Henna (L. inermis) on days 2, 4, 6, 8 and 10 post-injection

Injection days Fish group RBC x 106/mm3 Hematocrit (%) Hb (g/dl)

-2 Control (saline injected) 1.46 ± 0.22 39.2 ± 3.64 8.48 ± 1.3

Henna extract (6 mg kg-1 BW) 1.53 ± 0.18 38.4 ± 4.22 7.85 ± 0.88

Henna extract (60 mg kg-1 BW) 1.40 ± 0.23 38.6 ± 3.18 7.68 ± 0.77

Henna extract (600 mg kg-1 BW) 1.38 ± 0.33 38.2 ± 4.62 7.35 ± 1.2

2 Control (saline injected) 1.52 ± 0.26 39.8 ± 2.2 8.66 ± 0.56

Henna extract (6 mg kg-1 BW) 1.44 ± 0.20 38.3 ± 4.7 7.82 ± 1.3

Henna extract (60 mg kg-1 BW) 1.42 ± 0.28 40 ± 3.3 7.78 ± 0.61

Henna extract (600 mg kg-1 BW) 1.35 ± 0.36 38.2 ± 3.6 7.52 ± 1.14

4 Control (saline injected) 1.54 ± 0.28 42.6 ± 3.3 8.32 ± 0.56

Henna extract (6 mgkg-1BW) 1.44 ± 0.16 40.2 ± 3.1 7.20 ± 0.72

Henna extract (60 mgkg-1BW) 1.42 ± 0.18 39.3 ± 3.6 7.22 ± 0.83

Henna extract (600 mgkg-1BW) 1.36 ± 0.26 38.5 ± 4.4 7.55 ± 0.73

6 Control (saline injected) 1.56 ± 0.24 39.3 ± 3.3 8.28 ± 1.18

Henna extract (6 mgkg-1BW) 1.52 ± 0.19 39.6 ± 5.2 7.62 ± 1.12

Henna extract (60 mgkg-1BW) 1.42 ± 0.23 39.2 ± 3.4 7.53 ± 0.7

Henna extract (600 mgkg-1BW) 1.37 ± 0.27 38.6 ± 3.2 7.48 ± 1.14

8 Control (saline injected) 1.62 ± 0.24 42.3 ± 2.7 8.56 ± 0.68

Henna extract (6 mg kg-1 BW) 1.44 ± 0.18 39.3 ± 4.7 7.32 ± 1.24

Hennar extract (60 mg kg-1 BW) 1.39 ± 0.26 38.4 ± 2.6 7.85 ± 0.58

Henna extract (600 mgkg-1BW) 1.37 ± 0.33 38.8 ± 2.4 7.62 ± 0.64

10 Control (saline injected) 1.58 ± 0.21 39.5 ± 2.3 8.73 ± 0.58

Henna extract (6 mg kg-1 BW) 1.45 ± 0.34 38.3 ± 4.6 7.48 ± 1.12

Henna extract (60 mg kg-1 BW) 1.38 ± 0.26 39.4 ± 3.8 7.46 ± 0.79

Henna extract (600 mg kg-1 BW) 1.37 ± 0.28 38.2 ± 2.2 7.28 ± 0.64

Values are presented with the respective standard deviation (mean ± SD) (n = 6). Values in the same column showing the same superscript letter are not significantly different (p Tukey > 0.05)

Table 3 Effect of L. inermis (Henna) administration by intraperitoneal injection on relative percent survival (RPS) against LD50 concentration of A. hydrophila in common carp

Treatment Mortality (%) RPS (%)

Control (saline injected) 55.5 -

Henna extract (6 mg kg-1 BW) 44.4 20.0

Henna extract (60 mg kg-1 BW) 27.7 50.0*

Henna extract (600 mg kg-1 BW) 33.3 40.0*

RPS values with asterisk (*) differ significantly (p < 0.05) with control. Data expressed as mean ± SD (n = 18)

findings were obtained by Barrett (2003) and Widel et al. (2003), who reported that Echinacea preparations influenced the leukocyte count. Likewise, dietary garlic exhibited an increased level of WBC, lymphocytes, monocytes and neutrophils in C. carpio (Iranloye 2002). Furthermore, similar findings were observed in Cirrhinus mrigala fed with ginger and turmeric supplementations (Sivagurunathan et al. 2011) and in beluga (Huso huso) fed with garlic (Allium sativum) and nettle (Urtica dioica) supplemented diet (Nobahar et al. 2014). It is supposed that, increase in TLC especially in lymphocyte number may be in part due to the presence of flavonoids and terpenoids (Grayer et al. 1996; Lembberkovics et al. 1998; Sayyah et al. 2005) found in L. inermis.

Lymphocytes were functioned to produce antibody, to acknowledge and respond the antigen, and to be a mediator of cellular and humoral immune responses (Abbas et al. 2010). The significant increase in lymphocytes number in this study might also indicate the specific immunostimulatory role of L. inermis as previously reported for Echinacea purpurea (Aly et al. 2008).

Monocytes play important role in the defense system of fish body. They undergo transformation into macrophages and may be involved in phagocytosis and killing of pathogens upon first recognition and subsequent infections (Sivagurunathan et al. 2011). Monocytes have been reported to be sporadic in carp, tench, European catfish, rainbow trout, bream and perch (Mastoi et al. 2012). Nonetheless, in this study, a significant increased number of monocytes were recorded in the fish treated with medium or high dose of plant extract. In addition, the number of neutrophils was also increased. Neutrophils are the first cells to respond to infection within 24 h, increases during bacterial infections to phagocytose them (Sivagurunathan et al. 2011). Thus, increase in the TLC, neutrophils and monocytes in L. inermis extract treated fish can be attributed to the enhancement of non-specific immune responses, whereas increase in lymphocytes number may indicate a specific immune induction. These findings are supported with the results of previous investigations (Aly et al. 2008; Abdel-Tawwab et al. 2010; Sivagurunathan et al. 2012; Antache et al. 2014; Nobahar et al. 2014).

The presence of antimicrobial agents in fish blood can be evaluated by serum bactericidal activity and this is an important tool to analyze the innate immune system (Biller-Takahashi et al. 2013). In fact, independently of the effect of molecules and the mechanisms involved in the microbial killing, the measurement of the microbicidal activity is a very realistic approximation (Guardiola Abellan 2014). In this study, the increase in total serum protein and globulin level following herbal treatment, indicate the raise in protective proteins which can be correlated to the enhanced serum bactericidal activity (Ellis 1999; 2001; Magnadottir 2006; Maqsood et al. 2009). In this regard, a time course decreasing trend was observed in the number of bacterial colonies in the groups treated with either the medium or high dose of plant extract (Fig. 1j). The minimum number of bacterial colonies was recorded on day 10 post-treatment. Similarly, Quil-A, a fraction from Quillaja saponaria Molina, has enhanced serum bactericidal activity in Salmo gairdneri Richardson (Grayson et al. 1987). In addition, an increase in serum bactericidal activity in tilapia (Divyagnaneswari et al. 2008) in Indian major carp (Rao et al. 2006), in common carp (Alishahi and Abdy 2013) and in ornamental gold fish (Anusha et al. 2014) has reported after the administration of various herbal extracts.

For testing efficacy of an immunostimulant, it is very essential to estimate the increased protection in treated fish (Sakai et al. 2001). Current data revealed that mortality following challenge with A. hydrophila was decreased in the group of fish treated with either medium or high dose of herbal extract. There was an inverse relationship between the mortality rate and the level of extract administration. The enhancement of nonspecific immune parameters by L. inermis seed preparation is possibly an important factor in reducing the percentage mortality and thereby protecting the fish against live A. hydrophila challenge.

Earlier studies also revealed that dietary supplementation of Ocimum sanctum and Nyctanthes arbortristis leaves and intraperitoneal injection of water and hexane soluble fraction of Solanum trilobatum and Eclipta alba leaves enhanced the disease resistance against A. hydrophila in O. mossambicus (Logambal et al. 2000; Divyagnaneswari et al. 2008). This finding is in agreement with the results of Abutbul et al. (2004) in tilapia fed with a diet containing ethyl acetate extract of Rosmarinus officinalis leaf powder and where the disease resistance against A. hydrophila was enhanced in L. rohita fed with 0.5 % of Achyranthes aspera (Rao et al. 2006). Similar results were found in Carassius auratus fed crude extracts and purified fractions of Ixora coccinea incorporated in diet. Following challenge with highly virulent A. hydrophila AHV-1 the control diet fed fishes succumbed to death within 5 days at 100 % mortality whereas crude extracts and purified fractions fed groups survived 60 and 80 %, respectively, after 10 days (Anusha et al. 2014).

Mortality and relative percentage of survival (RPS) of common carp treated with henna extract and the control group after challenging with A. hydrophila is presented in Table 3. The RPS was highest (50.0 %) in medium dose treatment followed by high dose treatment (40.0 %) and was lowest (20.0 %) in low dose treatment. This might be due to the enhancement of the non-specific immune system of the fish by L. inermis. The RPS was strongly correlated with hematological studies and functional assays performed under the conditions of this study. These data are in agreement with the finding of Logambal et al. (2000) and Christybapita et al. (2007) in O. mossambicus, treated with O. sanctum and Eclipta alba leaf extract, respectively. Moreover, similar findings were obtained by an intraperitoneal administration of Solanum trilobatum Leaf extracts in O. mossambicus (Divyagnaneswari et al. 2008).

Collectively, it can be concluded that the protective ability of L. inermisis mediated through specific and non-specific immune mechanisms, as evident from the enhanced lymphocyte number and total immunoglobulin level as well as elevated phagocytic, NBT and lysozyme activities besides positive influence on haematological and biochemical parameters.

The results of the present investigation show that L. inermis methanolic extract can act as an immunos-timulant based on a time- and dose-dependent manner. Due to its effectiveness at low concentration, its use could be very cost effective. It is biodegradable and hence environment-friendly. Besides, L. inermis might have potential as an additive to fish feed. However, appropriate field trials remain necessary before using L. inermis extract as an immunostimulant in aquaculture.

Acknowledgments This study was supported by the Aquatic Animal Health and Diseases Department, School of Veterinary Medicine, Shiraz University through a research grant to S. Soltanian.

Open Access This article is distributed under the terms of the Creative Commons Attribution 4.0 International License (http://, which permits unrestricted use, distribution, and reproduction in any medium, provided you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made.


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