Potential Application of Lawsonia inermis L. (Lythraceae) Aqueous Extract as an Objectively Quantifiable Assay for Assessment of Viability of Protoscolices from Hydatid Cysts ()
1. Introduction
Cystic echinococcosis (CE), also known as hydatidosis, is a serious zoonotic disease of great public health and economic importance worldwide [1] . It is caused by infection with the metacestode larval stage (hydatid cyst) of the tapeworm Echinococcus granulosus senso lato, an intestinal parasite of canines, particularly dogs. The cysts develop in a wide range of domestic and wild ungulates as intermediate hosts and humans as an aberrant host following incidental ingestion of parasite eggs [2] . The definitive canine hosts acquire infection with the parasite when they ingest with viscera fertile hydatid cysts containing protoscolices (PSCs). A fertile hydatid cyst normally contains thousands of PSCs. Problems; however, arise on how to assess the infectivity of these PSCs in absence of a tangible method for measuring the success or failure of these PSCs to develop inside the canine host. Critical assessment of PSC infectivity would, therefore, be essential to determine the relative importance of different species of intermediate hosts in parasite transmission and epidemiology of the disease. In this respect, several studies adopted in vitro staining techniques for assessment of viability of PSCs (defined as capacity of being alive), a property closely linked to infectivity. Various chemical stains such as eosin [3] , trypan blue [4] or methylene blue [5] have been used for this purpose. There has been a remarkable increase of interest in natural product research over the past few decades for these products to be translated into practical applications in various fields such as medicine, agriculture, nutraceutical or cosmetics industries. Lawsonia inermis L. (Lythraceae), commonly called “Henna”, is a widespread plant universally famous for having dyeing properties [6] . It is commonly used for personal adornment especially body art and in industry. The plant has also been described to have medicinal benefits [7] [8] . Henna’s characteristic staining properties stem from the compound 2-hydroxy-1,4-naphthoquinone, known as lawsone; a red-orange pigment extracted from plant leaves [9] . The present study examines the potential application of aqueous extracts of L. inermis leaves for assessment of viability of PSCs from hydatid cysts taking uptake/exclusion of plant pigment as criteria.
2. Materials and Methods
2.1. Parasite Material
Hydatid cysts were recovered from the lungs of naturally infected camels slaughtered in a local market in Gezira State in Central Sudan. Intact cysts were transported to the parasitology laboratory at the Faculty of Veterinary Medicine, University of Khartoum. PSCs were recovered as a sediment following centrifugation of cyst fluid at 2000 rpm for 3 min at 25˚C.
2.2. Plant Extract
Crude, newly harvested L. inermis sun-dried leaves of 35 g were obtained from a local Sudanese market in Khartoum. They were soaked in distilled water to give a 12.5% w/v mix. The preparation was kept in a refrigerator at 4˚C for 24 hours and was subsequently strained through a fine mesh. Strained fluid was centrifuged at 2000 rpm for 3 minutes to obtain a clear working solution. The pH (3.13) was determined using pH meter (AD8000 Bench Meter, Adwa Instruments, Hungary) just before use.
2.3. Treatment
2 ml of the working solution was added to protoscolex sediment in a test tube. The tube was gently agitated with slight movements and the mixture was left to stand for 10 min, a period anticipated to enable the uptake or exclusion of plant pigment by PSCs. Contents were centrifuged at 1500 rpm for 2 min at 25˚C and the supernatant was discarded leaving a trickle of the working solution at the bottom of the tube. Samples were transferred with micropipettes to glass slides for microscopic examination. Control tests were performed with heat-killed PSCs [10] exposed to hot water at 60˚C for 3 min in a water bath. For comparative purposes, PSCs were treated with eosin 0.1% aqueous solution, a stain widely used for assessment of viability of PSCs [11] [12] . Imaging was performed with a digital camera (OPTICAM 4083. B1) fitted to an OPTICA Srl B-193 light microscope (Ponteranica, Italy), at magnification 100 and 400×.
2.4. Statistical Analysis and Interpretation of Results
The Echinococcus protoscolex has been described to have kinetically distinct molecular transfer systems for uptake of materials across the tegument (external body covering) [13] . Viability was assessed in terms of uptake/exclusion of plant pigments by viable (alive)/dead PSCs. Each of the experimental and control tests was replicated 5 times. Results were presented as frequencies of nominal variables in 2 × 2 contingency tables and analyzed by the Fisher exact probability test.
3. Results
Figure 1 shows the gross morphology of a non-stained Echinococcus protoscolex upon recovery from camel hydatid cyst showing the characteristic rostellar hooklets and calcareous corpuscles.
Normal PSCs exposed to L. inermis extract effectively excluded plant pigment when examined 10 min after exposure to extract (Figure 2(a), Figure 2(b)). No change in color could be observed between the PSCs as the test parasite and the surrounding extract medium.
In contrast, dead PSCs killed by heat before exposure to extract were permeable to the pigment acquiring the pigment distinctive color (Figure 3(a), Figure 3(b)). Frequencies for outcome of treatment (uptake/exclusion of plant pigment) were 0 and 5 for viable PSCs, respectively, as compared with frequencies of 5 and 0, in this order, for dead PSCs, respectively. This difference between viable and dead PSCs in response to treatment was statistically significant (p 0.0079).
Figure 1. Normal invaginated unstained Echinococcus protoscolex from camel hydatid cyst (400×).
(a) (b)
Figure 1. (a) Viable Echinococcus protoscolex following exposure to L. inermis leaves aqueous extract (400×); (b) Viable Echinococcus PSCs following exposure to L. inermis leaves aqueous extract (100×).
(a)(b)
Figure 3. (a) Dead Echinococcus protoscolex following exposure to L. inermis leaves aqueous extract (400×); (b) Dead Echinococcus PSCs following exposure to L. inermis leaves aqueous extract (100×).
Figure 4. Dead Echinococcus protoscolex exposed to eosin stain (400×).
Performance of the extract was comparable to that of eosin as evidenced by uptake of the stain by dead PSCs (Figure 4).
4. Discussion
Among parasitic helminths, tapeworms, having no digestive tract, nor a respiratory or a blood-circulatory system, utilize the tegument alone as a metabolically active body cover capable of performing vital functions such as digestion, absorption as well as protection of the parasite [14] [15] [16] . According to Pappas [17] , four distinct mechanisms, viz. pinocytosis, diffusion, active transport and facilitated diffusion, are implicated in nutrient uptake by tapeworms. The Echinococcus protoscolex, in particular, has been shown to have kinetically distinct molecular transfer systems for uptake of materials across the tegument [13] . Such properties enable the viability of PSCs to be assessed taking uptake/exclusion of materials as criteria. Results showed that viable PSCs invariably exclude L. inermis pigment in all 5 replicates. Control PSCs killed by heat, on the other hand, persistently acquire plant pigment. The actual mechanism by which a viable protoscolex excludes plant pigment and a dead protoscolex uptakes the pigment at the tegument cellular level, however, remains to be defined. It is proposed from the present study that application of L. inermis leaves aqueous extract has the potential to be employed effectively as a rapid, low-cost and an objectively quantifiable assay for assessment of viability of PSCs from hydatid cysts and that the distinction between viable and dead PSCs could be made in terms of exclusion or uptake of plant pigment, respectively.
5. Conclusion
Quantitative and qualitative analysis of the chemical composition of L. inermis leaves of Sudanese origin indicates presence of a multiplicity of components [18] . Further experiments are, therefore, necessary to standardize the method of assessment of viability by verifying the influence of such different components on the performance of the lawsone pigment as well the effect of the time of exposure to extract on PSCs.