|Year : 2011 | Volume
| Issue : 2 | Page : 279-284
The effect of Emblica officinalis diet on lifespan, sexual behavior, and fitness characters in Drosophila melanogaster
Pankaj Pathak1, BR Guru Prasad2, N Anjaneya Murthy3, SN Hegde4
1 Department of Basic Principles, JSS Ayurvedic Medical College and Hospital, Mysore, India
2 Department of Life Science, Kannada Bharthi College, Khusalnagar, India
3 AYUSH, Bangalore, India
4 Studies in Zoology, University of Mysore, Manasagangotri, Mysore, India
|Date of Web Publication||2-Feb-2012|
126/2, Abinanadan Jeweler, Vinoba Road, Shivarampet, Mysore - 570 001
Source of Support: None, Conflict of Interest: None
| Abstract|| |
Drosophila is an excellent organism to test Ayurvedic medicines. The objective of our study was to explore the potential of Emblica officinalis drug on longevity, sexual behavior, and reproductive fitness of Drosophila melanogaster using adult feeding method. Increase in the lifespan, fecundity, fertility, ovarioles number, and developmental time was observed in both parents and F1 generation, but not in the F2 generation in experimental culture (control + E. officinalis). According to the Duncan's multiple range test and ANOVA, there is a significant difference between two cultures. It was also noticed that E. officinalis influence some fitness characters in Drosophila along with sexual behavior.
Keywords: Ayurveda, Drosophila, Emblica officinalis
|How to cite this article:|
Pathak P, Guru Prasad B R, Murthy N A, Hegde S N. The effect of Emblica officinalis diet on lifespan, sexual behavior, and fitness characters in Drosophila melanogaster. AYU 2011;32:279-84
|How to cite this URL:|
Pathak P, Guru Prasad B R, Murthy N A, Hegde S N. The effect of Emblica officinalis diet on lifespan, sexual behavior, and fitness characters in Drosophila melanogaster. AYU [serial online] 2011 [cited 2019 Nov 20];32:279-84. Available from: http://www.ayujournal.org/text.asp?2011/32/2/279/92544
| Introduction|| |
Ayurveda literally "Science of Life"- is based on the twin principles of wholeness and balance. As a holistic healing tradition, Ayurveda recommends treating the "whole" person-body, mind, senses, emotions, and spirit instead of following the "one-cause-one-cure" principle and focusing on the symptoms of the moment. The premise on which this assumption is made is that if the roots are nourished and watered, the plant will flourish. Diet, sleep, lifestyle, daily and seasonal routines, and internal cleansing are just as, or more, important than herbs and potions in order to maintain good health. Ayurveda is equally about maintaining or preserving good health as it is about treating disorders--"Swaasthasya Rakshanam0"(Protection of health) is one of the goal of Ayurveda. 
The branch of rasayana or rejuvenation is one of the eight specialized branches of Ayurveda that primarily deals with the maintenance of health.  Rasayana is defined as any herb, food, or activity which confers youthfulness and cures diseases. If taken in a proper way, the rasayana prevents early aging and keeps person young and active, both physically and mentally.  The literal meaning of rasayana is "augmentation of rasa," the vital fluid produced by the digestion of food. Rasa provides nutrition, enhances the immunity, and sustains life. Rasayana is the method of treatment through which the rasa is maintained in the body. The purpose of rasayana is to give strength, immunity, ojus, vitality, will power, and determination, and to strengthen the sense faculties  so that you are not exposed to sickness and disease as long as you live.
According to Sushruta, sexuality and reproduction are so vital in Ayurveda that an entire discipline, known as Vajikarana, is dedicated to enhancing fertility and the rejuvenation of sexual and reproductive energy. Vajikarana therapy improves the function of the reproductive organs and vitalizes reproductive tissues, increasing semen count and strengthening their motility and making eggs more viable for conception. This not only enhances the quality and longevity of individual life, but also the health and vitality of offspring. Although some Vajikarana herbs work as aphrodisiacs, they also engender reproductive strength in order to increase the health of our offspring, or what vajikarana (aphrodisiacs) calls subahupraja. Emblica officinalis is such herb used as rasayana in treatment of diseases. However, effect of this drug on normal life activities has not been significantly validated. Therefore, the present study was carried out with an objective to explore the potential of E. officinalis drug on fitness of Drosophila melanogaster using adult feeding method. We have D. melanogaster as the test system which proved to be an excellent organism to test the effect of many drugs and other chemicals. 
The fruit fly Drosophila is one of the most intensively studied in medicine and serves as a model system for investigations of many developmental and cellular processes common to higher eukaryotes, including man. This fly is being used for genetic studies since almost a century. Studies on Drosophila have enabled biologists to make significant contributions to the fields as diverse as basic genetics, population biology, evolutionary biology, behavioral biology, and molecular biology. It has a short life cycle, easy and inexpensive in culturing, and they could be kept in large numbers. Library of several Drosophila species with mutant and transgenic stock is available at different laboratories in the world. Presence of giant polytene chromosome and less number of the chromosomes are added advantages of the flies for genetic studies. Its genome has also been sequenced recently.  Vertebrates have about four homologous for every gene found in Drosophila. The species shares large numbers of homologous genes with mammals, 13 601 with human beings. These have been analyzed to identify sequences related to those causing human diseases.  The evolutionary conservation of gene function between human beings and Drosophila make it an ideal model system for the study of the molecular mechanisms of human disease. Moreover, identification of specific genes that regulate life span in D. melanogaster has been achieved by two processes: I. mutational analysis,  in which manipulation of pathway function or gene has demonstrated life span extension, and II. Quantitative trait locus analysis,  in which genetic elements affecting natural variations in longevity have been mapped to specific positions along the chromosomes. , In Drosophila and many other insects, body size is positively correlated with mating success, longevity, fecundity, and other fitness characters and best phenotypic heritable characters.  All these findings demonstrated the advantage of size in mating success and fitness. Various workers demonstrated the fitness studies in Drosophila such as fecundity, fertility,  and longevity. ,
Survey of the literature shows  on decrease gene activity such as chico, dlip genes, dS6K, dTOR, DTS-3. EcR. Indy, InR, mth, ovo, Puc extends the lifespan in D. melanogaster. Simultaneously, there are genes such as Cat CCtl dFOXO, DPOSH, dTSc1, dTSc2, EF-1a, fwd, G6PD, magu, Mel-41, Pcmt, and PTEN which increase gene activity leads to lifespan extends. Moreover, with these genes (Catsup, Ddc, Dox-A2, Lim 3, stc), allelic variation also varies longevity of fruit flies. These facts have shown that D. melanogaster is one of the most excellent eukaryote for exploring the genetic determination of life span, genetics of degeneration and aging process, and reproductive capacity. With these results, there is an insight into what to seek in man. For instant, the human Xist gene and the analogous Drosophila Sxl gene both control sex determination, and may both be involved in regulating longevity. This shows that any investigation of E. officinalis on the aging process on Drosophila will be fruitful research. In order to validate E. officinalis concepts more precisely, we proposed using D. melanogaster as a model. Till now, not much literature is available for evaluation of Ayurvedic medicine on life span on Drosophila. E. officinalis fruit is one of the Ayurvedic drug used in Rasayana Chikitsa. Ayurveda lexicons state that the fruit of E. officinalis is the best medicine to increase the lifespan. The biological effect of this drug has not been tested in recent times, especially in Drosophila, but only is being prescribed to human beings. Furthermore, assessing its effect in human beings has practical and ethical problems. Therefore, to revalidate the concept of Rasayana Chikitsa and in particular to assess the effect of E. officinalis, the present study has been carried out using D. melanogaster as the test system. A rasayana from E. officinalis was formulated based on the traditional principles; this is carefully altered to reflect intrinsic differences between mammals and insects. Here, we tried to investigate the impact of the E. officinalis on fitness parameters such as number of fertility, fecundity, ovarioles, and developmental time in D. melanogaster flies and in next generation along with sexual behavior.
| Materials and Methods|| |
Preparation of cultures
To study the impact of E. officinalis on some quantitative sexual behavior and fitness parameters, D. melanogaster (Mysore strain) flies were obtained from Drosophila stock center, Department of Zoology, Mysore, and were used in the present study. The pure culture of these flies was maintained under standard food medium.  The effect of E. officinalis was studied by adult feeding method. For this purpose, the stocks of the flies were built up for five to six generation from isofemale line. The virgin females and bachelor males that emerged from the normal media were isolated under ether anesthesia within 3 hours of eclosion. They were transferred to 8 × 2.5 cm glass culture vials containing equal quantities of normal food media used for Drosophila culture (wheat cream agar medium--this medium was prepared by boiling 1 000 ml of distilled water along with 100 g of jaggery [sugar]. When jaggery was dissolved in it, 100 g of wheat powder [soji or rava] was added to the medium and then 10 g of agar agar and 7.5 ml of propionic acid [antifungal] were added gently). The medium was distributed to glass vials of 8 × 2.5 cm size. The mouth of the bottles/vials was kept closed with cotton. One day later, one or two drops of yeast solution were added to the food media. This medium was used after 24 hours. At every step, heat vials were used for preparing medium. This was to prevent outbreak of pests and diseases. Similarly, sterilized cotton was used to plug the vials. This culture is used as control culture. For experimental culture, 5 drops of E. officinalis was included to the above wheat cream agar medium and virgin females and bachelor males were transferred into this media and aged for 4 days. There was no dietary restriction for the flies in both control and experimental culture.
For longevity (life span), 25 virgin females and bachelor males from both cultures were used to test the longevity. For this purpose, each pairs were transferred to control culture and experimental culture. Daily, these flies were transferred to the fresh vials of both cultures until flies die from the day of eclosion. This is calculated in terms of number of days.
For analysis of sexual behavior patterns, 50 virgin females and fifty bachelor males that emerged from the normal media were isolated under ether anesthesia within 3 hours of eclosion and maintained them separately in both control and experimental culture for 4 days. Twenty-five flies of both the sex were used to study some courtship activities, , such as mating latency, copulation duration. For observation of sexual behavior, a virgin female and bachelor male were introduced into an Elens-Wattiaux mating chamber (5 × 5 cm circular glass chamber with a lid to facilitate easy observation). Because maximum mating occurs during morning hours, observation was made between 7 and 11 a. m. Mating latency (time between introduction of males and females into mating chamber and initiation of copulation of each pair) and copulation duration (time between initiation and termination of copulation of each pair) were recorded. The terminologies are used as per the description of Hegde and Krishnamurthy.  A minimum of 25 pairs involving each isofemale line were observed for both culture groups. Similarly, mating latency and copulation duration was also observed in the F1 generation and F2 generation (fed with normal food media), which were generated from the above 25 mated pairs which are considered as parents.
The reproductive fitness parameters such as fecundity, fertility, ovarioles number, and developmental time were analyzed from mated parents and their two successive generations. For fecundity test, mated males were transferred to vials containing normal food media and allowed to lay eggs for 24 hours. After 24 hours, the flies were individually transferred to fresh vial containing food media. The number of eggs laid (fecundity) during the following ten days was scored using stereomicroscope for both control and experimental groups. Twenty-five replicates were maintained for each of the control and experiment studies. The fertility was measured by counting the number of the progeny produced by a single mated female. For testing fertility, each mated female was kept in an individual food vial for a period of one day and then transferred to a fresh food vial every day. Ten successive changes were made and the total number of flies that emerged from each vial was counted. Twenty-five replicates were maintained for each of the experimental and control under study. Data were pooled and the mean number of flies per female was calculated. Counting of ovarioles number was done by selecting the 25 virgin females separately and maintained in both control and experimental cultures and aged for 4 days. These virgin females were dissected for left ovaries in saline and bundles of ovarioles were separated by fine needle and counted under a stereomicroscope. For analysis of developmental time, after emergence of the flies were counted every day from the first to last day of the eclosion. A minimum two pairs of virgin female and bachelor's male were selected from all 10 vials which are considered as F1 generation. Similarly, for F2 generation, flies were selected from the F1 generation. These were mated separately maintained in the separate vial to calculate their fecundity, fertility, developmental time, and ovarioles number too. All the culture was maintained under the laboratory condition at a temperature 24 ± 2°C. One way analysis of variance (ANOVA) followed by Duncan's multiple range test (DMRT) was applied for all parameters using SPSS 10.5 software.
| Results|| |
The data on the longevity (lifespan) presented in [Table 1] reflect longevity of D. melanogaster where the parent flies fed with experimental culture shows high lifespan with mean value 76.8 ± 40.6 than F1 generation (70.3 ± 15.3), F2 generation (57.3 ± 15.4) with F value = 147.36 and control one (41.9 ± 14.0; F1 generation (40. 2 ± 12.0); F2 generation (42.0 ± 20.9) with F value = 27.2.
The data on sexual behavior and fitness parameters of D. melanogaster of two different cultures have been reported in [Table 2]. Sexual activities such as mating latency was highest in control culture than experimental culture (10.32 ± 0.72) and it is significant by one way ANOVA and DMRT (F value = 20.04; P < 00.001) between the two cultures; this is also seen in their successive generations. Meanwhile, copulation duration is highest in experimental culture (28.64 ± 1.15) compared with control culture. This prolongation of copulation was also observed in the next generation.
The scrutiny of [Table 2] shows that fitness parameters such as fecundity, fertility, developmental time, and ovarioles number was high in experimental culture compared with control and significant too between two cultures (fecundity = 131.1 ± 1.36, fertility = 122.9 ± 1.32, developmental time = 15.63 ± 0.15, ovarioles number = 17.00 ± 0.73, F value = 24.85; 16.73; 6.57; 15.75; these mean values are more compared with their F1 and F2 generations. [Table 2] presents mean values of fitness parameters, where F1 progeny shows high values compared with F2 generation (Fecundity = 128.1 ± 1.21, fertility = 120.3 ± 1.47; developmental time = 14.04 ± 0.13; ovarioles number = 15.00 ± 0.71). All these parameters are highly significant when comparison is done between the cultures [Table 2]. The above fitness parameters and sexual behavior are depicted in [Figure 1] and [Figure 2], where flies reared in control media show no such variation among the parameters, but there is variation in the mean values in the experimental culture between the parents, F1 generation, and F2 generation.
|Figure1: Fitness parameters and sexual behavior of Drosophila melanogaster cultured in control media (units; fecundity, fertility, developmental time, ovarioles = numbers, copulation duration = minutes; mating latency = seconds)|
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|Figure2: Fitness parameters and sexual behavior of Drosophila melanogaster cultured in experimental media (Control + Emblica officinalis) (units; fecundity, fertility, developmental time, ovarioles = numbers, copulation duration = minutes; mating latency = seconds)|
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| Discussion|| |
For the above results, the longevity is more in case of parents compared with their progenies in experimental culture-fed flies than control one; this confirms that there is an influence of E. officinalis which is mixed in experimental culture. These results validate the statement of Acharya Charaka which says "Amlakah vayah sthapananam sreshtha"  (Fruit of E. officinalis is the best to increase the longevity). Sexually reproducing animals are endowed with special features, first to produce fertile offspring and second to adapt to a particular environment. The reproduction is preceded by a series of courtship acts wherein males and females show unique rituals to attract each other, mate, and produce the offspring. The courtship and mating although are genetic, are also influenced by various factors. This may imply that these courtship activities are directed by the same set of genes and that these traits are related genetically. This agrees with the observations which show the genetic determination of certain components of sexual behavior in Drosophila.,, Though genetically determined, there is every possibility for a change in sexual behavior because these activities are also influenced by changes in physical environment. ,,,, In the present study, an effort is made to study the effect of E. officinalis on quantitative sexual behavior and fitness parameters.
The data obtained from our studies show that the mating latency was shorter in the flies reared in experimental culture in comparison with control [Table 1]. The differences in mating latency in two cultures were also statistically significant (by ANOVA and DMRT). Mating latency is measured as the time taken for the male oriented toward female until initiation of copulation duration by Markow.  It is the period during which the pairs acclimatize in the mating chamber and then start the courtship activities. It actually indicates the vigor of male.  A male with high vigor reacts quickly in the presence of female, whereas a male with less vigor reacts slowly. , Obviously shorter mating latency indicates higher vigor of male. The shorter mating latency was noticed in experimental culture. This suggests that the males from experimental culture have higher vigor and therefore are quickly attracted by the females. The mating latency was also shorter in the flies from experimental culture compared with control shown in [Figure 1] and [Figure 2]. The mating latency not only indicates vigor of males, but also receptivity of females. It is the time required for males and females to initiate copulation. Higher the vigor of males and receptivity of females, shorter is the mating latency. During this period, courtship acts are performed mostly by males, to increase the receptivity of females and to make her sexually excited.  A male with high vigor has to perform the same courtship act more number of times to a nonreceptive female than to a receptive female. If she is receptive, only a few courtship acts are performed leading to quick pairing. The short matinglatency of experimental culture in the present study indicates that the males maintain high vigor and females maintain high receptivity at this culture, while those in control could not maintain the vigor and receptivity. Mating latency of control culture of parents and their generations are more or less equal [Table 2].
Courtship activity of the male or female culminates in copulation demonstrated by Spiess.  During copulation, sperms from the male is transferred to the female reproductive tract and therefore the duration of copulation has a lot of significance in an animal's life. In the present study, the copulation duration was longest in flies maintained on experimental culture than those maintained on control culture. According to Guruprasad et al.,  longer duration of copulation permits the transfer of more number of sperms by male to the female. Therefore, extension of copulation duration enhances the fitness of the male. It can also enhance the fitness of the females because the sperms received by a female can fertilize more number of eggs. Therefore, it is unlikely that the longer copulation duration could enhance the fitness, as the females have high receptivity and males have high vigor.
In Drosophila, the fecundity remains one of the less-known quantitative traits along with fitness parameters such as fertility, developmental time, and ovarioles number. Estimation of fecundity and fertility is important in routine testing of various chemicals. This gives an insight into the extent of effect on ovarioles and other physiological factors, which is expressed in the terms of egg and offspring production. [Table 2] reveals that the mean fecundity eggs/female in the adult feeding methods was more than control. ANOVA and DMRT analyses have shown that increased fecundity in experimental culture reared flies were significant (P < 00.001). This indicates that the mode of administration is also important factor, which one should consider while assessing the effect of any chemical on any biological system. In contrast to this, in control culture, the decrease in fecundity may be accounted for the fact that the flies are under the influence of E. officinalis; hence, they might not have been able to lay eggs rather than producing less egg. This finding agrees with the observation  where they noticed oviposition rhythm in D. melanogaster, and Vogel  has demonstrated that certain aziridine analogs have discernible effect on fecundity in Drosophila. [Table 1] also incorporates that mean fertility per female in adult experimental diet with E. officinalis significantly increases when compared with control, and they were more fertile than control, (P < 0.001 by ANOVA and DMRT). Several workers have made studies on the effect of different chemicals on fertility in D. melanogaster. The present study agrees with them that influence of the chemicals will alter the fertility in Drosophila.
Rate of development is another parameter, which is used to evaluate some chemicals clinically. In the present investigations, the genetic constitution, amount of the food, temperature, and space were kept constant. Obviously, the differences in the development must have been determined by the chemical used or not by the other factors. This type of effect on the developmental time by different chemicals in D. melanogaster. is well known.
The estimation of fitness is the first step in understanding the adaptive evolution of a population. Ovariole number is an anatomical trait determined during pupation for which a polygenic basis is known in various species of the D. melanogaster complex. Interestingly, our results are contrary to this where experimental culture-fed flies are having more ovarioles than control; this shows that there is influence of the E. officinalis rasayana mixed in experimental culture.
[Figure 1] suggests that all the fitness parameters and sexual behavior of D. melanogaster reared in control media is similar in all parents and their generation too. According to [Figure 2], fitness parameters and sexual behavior of D. melanogaster in experimental media have variation among F1 generation and F2 generation compared with their parents. The Flies which are fed with the experimental culture have long life span than control one [Table 1]. Our results confirm the effect of E. officinalis on parents than their progenies and the impact of E. officinalis is carried to F1 generation rather to F2 generation in experimental culture.
| Conclusion|| |
The data generated in this study showed variation in the developmental time in both cultures [Table 2]; longest mean of developmental time was noticed in the experimental cultures. The conclusion of our experiment suggests that E. officinalis enhances the sexual activities. This obviously increases longevity, fertility, fecundity, ovarioles number along with developmental time. Finally, it is inferred that there is a linear interrelationship between sexual activities and fitness parameters in experimental culture. "Adding Life to years is better than adding years to life." So, along with longevity, other reproductive fitness characters of flies were considered for this study so as to explore the hidden principles of Rasayana therapy which improves the quality of the life.
| References|| |
|1.||Agnivesha, Charaka, Dridabala, Charaka samhita, Sutra sthana Arthedasha mahamooliye Adhyaya, 30/26. Vaidya Yadavji Trikamji Acharya, editor. 5 th ed. Varanasi: Chowkamba Orientalia; 2001. p. 187. |
|2.||Sushruta, Sushruta samhita, Sutra sthana Vedotpatti Adhyaya, 1/8. Vaidya Yadavji Trikamji Acharya, editor. 7 th ed. Varanasi: Chowkamba Orientalia; 2002. p. 26. |
|3.||Ibidem Charaka Samhita , Rasayana Chikitsa Adhyaya, 1/7.2001. p. 376. |
|4.||Ibidem Charaka Samhita , Rasayana Chikitsa Adhyaya, 1/11, 2001; p. 377. |
|5.||Mansour N, Hegde SN. Effect of Flouxetine on the courtship latency, mating latency and copulation duration of Drosophila melanogaster. J Pakistan Med 2006;90:58-63. |
|6.||Adams MD, Celniker SE, Holt RA, Evans CA, Gocayne JD, Amanatides PG, et al. The Genome sequence of Drosophila Melanogaster. Science 2000;287:2185-95. |
|7.||Reiter LT, Potocki L, Chein S, Ghribskov M, Bier E. A systematic analysis of human disease-associated gene sequences in Drosophila melanogaster. Genome Res 2001;11:1114-25. |
|8.||Ford D, Tower J. Genetic manipulation of lifespan in Drosophila melanogaster. In: Masaro EJ, Austad SN, editors. Hand book of the Biology of aging. 6 th ed. Burlington, MA: Elsevier Press; 2006. p. 400-14. |
|9.||Tatar M, Yin C. Slow aging during insect reproductive Diapause: Why butterflies, grasshoppers and flies are like worms. Exp Geronotol 2001;36:723-38. |
|10.||Paaby AB, Schmidt PS. Functional significance of allelic variation at methusselab, an aging gene in Drosophila. Plos One 2008;3: e1987. |
|11.||Paaby AB, Schmidt PS. Dissecting the genetics of longevity in Drosophila melanogaster. Fly 2009;3.1:29-38. |
|12.||Santos M, Ruiz A, Quezada-Diaz JE, Barbadilla A, Fontdevila A. The evolutionary history of Drosophila buzzatii. XX. Positive phenotypic covariance between field adult fitness components and body size. J Evol Biol 1992;5:403-22. |
|13.||Long CE, Markow TA, Yaeger P. Relative male age, fertility, and competitive mating success in Drosophila melanogaster. Behav Genet 1980;10:163-70. |
|14.||Cordts R, Partridge L. Courtship reduces longevity in male Drosophila melanogaster. Anim Behav 1996;52:269-78. |
|15.||Partridge L, Tower. Yeast a Feast: The Fruit fly Drosophila as a model organism for research in aging. Moleular Biology of Aging. In: Garanto L, Partridge L, Wallace D, editors. Cold Spring Harbor: Cold spring Harbor laboratory press; 2008. |
|16.||Guruprasad BR, Hegde SN, Krishna MS. Seasonal and altitudinal variation of 20 Species of Chamundi hill. J Insect Sci 2010;10:123. |
|17.||Spieth HT, Ringo JM, Mating behavior and sexual isolation in Drosophila. In the genetics and biology of Drosophila. Ashburner M, Carsony HL, Thompson Jr JN, editors. Vol. 3c. London; Academic Press; 1983. p. 223-4. |
|18.||Hegde SN, Krishnamurthy NB. Studies on mating behavior in the Drosophila bipectinata complex. Aust J Zool 1979;27:421-31. |
|19.||Ibidem Charaka samhita (1). Yagnyapurshiye Adhyaya, 25/40.2001;p. 132. |
|20.||Charaka Samhita Sutrasthana. Bhagvan Dash Vol. 1, 6 th edition. Chowkambha series office, Varanasi, India: Chowkamba Orientalia; 2000;25:17,2000. |
|21.||Spiess EB. Mating propensity and its genetic basis in Drosophila. In essay in evolution and genetics in honour of the Dobzhansky. Hecht MT, Streere WC, editors. New York: Appleton-Century- Crafts; 1970. p. 315-79. |
|22.||Parsons PA. Behavioral and Ecological genetics: A study in Drosophila. Oxford: Clarenden Press; 1973. p. 1-55. |
|23.||Crossley SA. Changes in mating behavior produced by selection for the ecological between and vestigial mutants of Drosophila melanogaster. Evolution 1974;28:631-47. |
|24.||Gutzke WH, Crews D. Embryonic temperature determines adult sexuality in a reptile. Nature 1998;332:832-4. |
|25.||Laudien H, Fecher W, Schumann W. Temperature dependence of Courtship in male guppies, Poecilia reticulate. Peters (Pisces, Cyprinidae). Z Tieropaychol 1980;52:1-18. |
|26.||Sisodia S, Singh BN. Effect of the temperature on longevity and trade productivity in Drosophila ananassae; evidence for adaptive plasticity and trade off between longevity and productivity. Genetika 2002;114:95-102. |
|27.||West PM, Packer C. Sexual selection, temperature and the lion's mane. Science 2002;297:1339-43. |
|28.||Markow TA. A comparative investigation of the mating system of Drosophila hydei. Anim Behav 1985;33:775-81. |
|29.||Eastwood L, Burnet B. Courtship latency in male D. malenogaster. Behav Genet 1977;7:359-72. |
|30.||Markow TA. Reproductive behavior of Drosophila melanogaster and Drosophila nigra spiracula in the field and in the laboratory. T Comp Pshycol 1988;102:169-73. |
|31.||Guruprasad BR, Hegde SN, Krishna MS. Positive correlation between male size and remating success in few populations of D. bipectinata, Zoological studies 2008;47:75-83. |
|32.||Gruwes G, Hoste C, Lints CV, Lints FA. Oviposition rhythm in Drosophila melanogaster and its alteration by change in the photoperiodicity. Experientia 1971;27:1414-6 . |
|33.||Vogel E. Differential sensitivity of immature and mature oocytes of Drosophila melanogaster to the induction of dominant lethals following treatment by mono-polyfunctonal azaridine analogues. Mutat Res 1972;14:250-3. |
|34.||Vasudeva V, Krishnamurthy NB. Effect of Dithane M-45 on the rate of development, viability, morphology, and fecundity in Drosophila melanogaster. J Mysore Univ 1983;29:79-86. |
|35.||Luning KG. Drosophila tests in pharmacology. Nature 1966;209:84-6. |
[Figure 1], [Figure 2]
[Table 1], [Table 2]