Descriptions of the developmental stages of embryonic marine turtles are presented in the form of a dichotomous key supported by drawings to facilitate identifying stages of development in the field. The key emphasizes the sequential appearance or loss of external morphological structures that can be seen either with the unaided eye or with a ×10 hand lens and a handheld light. Stages are placed in the context of normal beach temperatures to facilitate estimation of laying date, emergence date, and events that cause embryonic mortality. Measurements of embryos are presented to assist determining stage.
The earliest descriptions of marine turtle embryos were made from specimens collected opportunistically to illustrate specific aspects of development. For example, embryos obtained at different times during development were described and illustrated for Eretmochelys imbricata (Voeltzkow 1903; Fuchs 1915; Deraniyagala 1939), Chelonia mydas (Parker 1880; Deraniyagala 1939; Penyapol 1958; Domantay 1968), Caretta caretta (Agassiz 1857; Mitsukuri 1894, 1896–1898; Jordan 1917; Fujiwara 1966; Kondo 1986; Kuratani 1999), Lepidochelys olivacea (Deraniyagala 1939), and Dermochelys coriacea (Deraniyagala 1933, 1939, 1953) as part of a variety of studies. Agassiz (1857), Mitsukuri (1894, 1896–1898), and Fujiwara (1966, 1971) examined aspects of ovipositional development. Raynaud et al. (1980) focused on the projections of the epithelia of the branchial arches of leatherback turtles (D. coriacea). Kuratani (1999) described the development of the chondrocranium in C. caretta embryos. Billett et al. (1992) used scanning electron microscopy to enhance the descriptions of C. caretta embryos. None of these studies provided a complete developmental sequence for any species of marine turtle.
The first standard developmental sequence for a marine turtle from oviposition to hatching was produced by Crastz (1982) for L. olivacea. Miller (1985b) combined descriptions of embryos of the Cheloniidae to define developmental stages from fertilization through preemergence for all species of marine turtles. More recently, Kaska and Downie (1999) used Miller's postovipositional stages to describe green and loggerhead turtle embryos in the Mediterranean. Embryonic development of the leatherback was described in detail by Renous et al. (1989) based on Miller (1985b). Al-Mukhaini et al. (2010) used Miller's definitions as a foundation to describe development in green turtle embryos at 30°C.
PRACTICAL APPLICATIONS OF A STAGING KEY
Staging tables provide a description of ontogenetic changes of embryos incubated under defined conditions (Hamburger and Hamilton 1951; Ewert 1985; Miller 1985a; Hopwood 2007) that can be used to assess development under various conditions, such as natural, experimental, and unknown (e.g., C. caretta, Özdemir et al. 2008; Carettochelys insculpta, Beggs et al. 2000; Crocodylus porosus, Magnusson and Taylor 1980; Webb et al. 1983).
Embryonic development occurs within the complex environment of the nesting beach (Ackerman 1997). As a result, nest site selection has a significant impact on incubation because the environment experienced by the developing embryos depends on the location selected by the nesting female (Mortimer 1982; Wood and Bjorndal 2000; Miller et al. 2003; Serafini et al. 2009). The physical characteristics of the substrate mediate thermal and hydric insulation and gas exchange between the environment and the developing embryos within the nest (Mortimer 1990; Ackerman 1997; Hewavisenthi and Parmenter 2002; Ackerman and Lott 2004).
Field assessment of the stage and time during incubation at which embryos died can help to identify mortality factors, such as subsand flooding (Caut et al. 2010), excessive rainfall (Ragotzkie 1959), inundation (Foley et al. 2006), collapse of egg chambers during pipping and hatchling emergence (Mortimer 1990), and extreme temperatures (Valverde et al. 2010), that affect embryonic survival in the nesting beach. Herein we present a simplified key to developmental stages of marine turtles, which in conjunction with knowledge of beach temperature and/or duration of incubation, helps bracket when mortality occurred, thereby helping to identify mortality factors.
METHODS USED TO GENERATE THE KEY
Miller (1985b) defined 31 stages in the development of marine turtle embryos, of which stages 1–5 occur inside the oviduct of the female and stages 6–31 occur in the nest after oviposition. The five preovipositional stages described by Miller (1985b) are not included in the key. For stages 6–31, only those external morphological characters that can be seen by the unaided eye or by using a ×10 hand lens and a handheld light are presented in the key. The original stage descriptions were a composite compiled from examination of multiple individuals of each species incubated under natural and controlled conditions (Miller 1982, 1985b). Descriptions of characters that relate to only one species have been de-emphasized in favor of general ones that place the specimen in an appropriate stage regardless of species. Drawings were made from specimens and photographs. Volume of embryos and their yolks was determined by water displacement in a graduated cylinder (± 2.5 cc). Measurements were made using Vernier calipers (± 0.1 mm) on fresh and preserved specimens.
Eggs were collected at oviposition and moved to a protected hatchery area or into incubators (temperatures: 26°C ± 0.5°C, 29°C ± 0.5°C, 32°C ± 0.5°C). The majority were moved within 1 hr (Limpus et al. 1979). Eggs of C. mydas, Natator depressus, C. caretta, and D. coriacea were incubated under both laboratory and beach conditions; eggs of other species were incubated in beach hatcheries (Miller 1982). The L. olivacea embryos examined were unhatched remnants of emerged clutches; these specimens were compared with descriptions by Crastz (1982) to assign appropriate stages.
In the following key, the chronology of the stages is given as a percentage of the developmental time based on eggs incubated at 29°C. Although not providing exact timing of when a stage occurred, the use of a percentage accommodates variation in the duration of development at different temperatures under field conditions. The use of 29°C as the baseline is justified because the temperature is 1) near the middle of the embryonic tolerance limits (Ackerman 1997) and 2) near the pivotal temperature for sexual differentiation for most species (except for Lepidochelys) (Wibbels 2003).
Measurements of specific characteristics are presented by species to augment the determination of a stage. Total disc length was measured as the straight distance between the anterior and posterior of the embryonic disc; crown-to-rump length was measured as the straight distance from the top of the curled embryo to the curl at the base of the tail. Forelimb length was measured as the straight distance between the proximal and distal ends of the flipper manus of the developing embryo. Straight carapace length was measured as the straight distance between the anterior and posterior ends of the carapace of the developing embryo. Straight carapace width was measured as the straight distance across the carapace of the developing embryo. Interclaw distance was measured as the straight distance between the claws of the fore flipper. Development time is defined as the interval from oviposition to pipping. Pipping takes place when the embryo ruptures the eggshell. Hatching occurs when the embryo exits the eggshell. Emergence is defined as when the hatchling appears on the beach surface.
RESULTS: THE KEY
The following dichotomous key to the stages of development of the Cheloniidae (and in general to development of Dermochelys) (Figs. 1 and 2) is based on developmental stages defined by Miller (1985b), using embryos of C. mydas (n = 733), N. depressus (n = 375), C. caretta (n = 1303), Eretmocheleys imbricata (n = 567), L. olivacea (n = 51), and Dermochleys coriacea (n = 96) (Miller 1985b).
Dichotomous Key to the Embryonic Stages of Marine Turtles when Eggs Have Been Removed from a Nest on the Beach or Other Conditions of Incubation
(Based on developmental stage definitions by Miller 1985b. %DT [development time] = % of incubation time from oviposition to pipping for eggs incubated at 29°C.)
1a. Embryo recognizable as a turtle with pigment on the carapace23
1a. Embryo other than with pigmented carapace2
2a. Embryo with limbs twisted flat against the sides of the body and with iris pigmentation21
2b. Embryo other than above3
3a. Embryo with definite head and eyes and with laterally projecting limb buds17
3b. Embryo other than above4
4a. Embryo mostly disk shaped, lacking eye bulges5
4b. Embryo elongate with definite eye bulges13
5a. Blastopore shaped as a transverse slit or as a wide, anteriorly opening crescent Oviposition Stage 6 [0.5 ± 0.5 %DT]
5b. Embryonic area not as above6
6a. Blastopore shaped as a posteriorly opening crescent Stage 7 [1.2 ± 0.5 %DT]
6b. Embryonic area not as above7
7a. Blastopore shaped as an inverted “U”; head fold indicatedStage 8 [2.8 ± 0.5 %DT]
7b. Embryonic area not as above8
8a. Blastopore shaped as an inverted “U”; head fold shaped as a posteriorly opening crescent; no somites presentStage 9 [3.8 ± 0.5 %DT]
8b. Not as above9
9a. 2 or 3 pairs of somites present; neural crests touch at posterior end of headStage 10 [4.8 ± 0.5 %DT]
9b. More than 4 pairs of somites present10
10a. 5 or 6 pairs of somites present; neural crests touching or fusing along midline of head Stage 11 [5.7 ± 0.5 %DT]
10b. More than 6 pairs of somites present11
11a. 8–10 pairs of somites present; amnion covers about one-half of the total lengthStage 12 [6.7 ± 0.5 %DT]
11b. More than 11 pairs of somites present12
12a. 12–14 pairs of somites present; neurocentric canal bounded posteriorly by a low ridge; amnion covers about three-fourths of total length Stage 13 [7.6 ± 0.5 %DT]
12b. More than 14 pairs of somites present13
13a. 15–17 pairs of somites present; mouth not open; amnion covers neurocentric canal Stage 14 [8.6 ± 0.5 %DT]
13b. More than 17 pairs of somites present14
14a. 19–21 pairs of somites present; mouth open as a deep “V”; first pharyngeal cleft open; posterior amnionic tube formedStage 15 [11.5 ± 1 %DT]
14b. More than 21 pairs of somites present15
15a. 23–25 pairs of somites present; lens differentiated in the eye, pharyngeal clefts 1 and 2 open; small limb buds visible on lateral body wall Stage 16 [13.4 ± 1 %DT]
15b. More than 26 pairs of somites present16
16a. 29–34 pairs of somites present; limb buds bulge lateroposteriorly; all pharyngeal clefts open Stage 17 [16.3 ± 1 %DT]
16b. More than 35 pairs of somites present17
17a. 35–40 pairs of somites present; digital plates not free of body wall; flaps have developed on anterior borders of all pharyngeal cleftsStage 18 [19.2 ± 1 %DT]
17b. More than 40 pairs of somites present18
18a. 40–45 pairs of somites present; digital plates free from body wall and project laterally Stage 19 [22.0 ± 1 %DT]
18b. More than 45 pairs of somites present19
19a. Digital plates partially or completely twisted flat against the body wall; iris unpigmented; pharyngeal clefts nearly closedStage 20 [25.0 ± 1 %DT]
19b. Not as above20
20a. Iris pigmented along its posterior border; carapace rudiment is a ridge on the lateral body wall and extends above the bases of the limbs; digital plates without serrations; digital plate not separated from limb by a ridgeStage 21 [29.5 ± 1 %DT]
20b. Not as above21
21a. A distal ridge defines the limit of the limb from the digital plate; marginal ridge of carapace marked by small, low serrations; pharyngeal clefts closed Stage 22 [34.5 ± 1 %DT]
21b. Not as above22
22a. Posterior border of carapace complete at least by a low ridge; anterior border incomplete; digital serrations present indicated as shallow ridges and grooves Stage 23 [39.4 ± 1 %DT]
22b. Not as above23
23a. Anterior border of carapace indicated by at least a low ridge across neck; posterior border of inframarginal area is defined; anterior is not; scutes of carapace indicated; flecks of pigmentation may occur on carapace; digital serrations present as ridges and grooves.Stage 24 [45.0 ± 1 %DT]
23b. Not as above24
24a. Periphery of carapace complete anteriorly and posteriorly; all scutes have differentiated; body and flipper scales undifferentiated; tagging scales may be indicated; digital serrations elongate; claw rudiment presentStage 25 [53.0 ± 2 %DT]
24b. Not as above25
25a. Scutes of carapace becoming pigmented; head scales, except over ear, and cutaneous papillae present; all flipper scales present; tops of scales may be pigmented; tagging scales presentStage 26 [62.0 ± 2 %DT]
25b. Not as above26
26a. Unpigmented scales over ear region except pigmented in hawksbill; all flipper scales present and pigmented; transverse plastronal fold indicated as a bend perpendicular to axis of body; yolk volume greater than specimenStage 27 [70.6 ± 2 %DT]
26b. Not as above27
27a. Scales over ear pigmented; transverse plastronal fold forms oblique angle between abdominal and thoracic scutes; specimen volume about equal to yolk volumeStage 28 [78.3 ± 2 %DT]
27b. Not as above28
28a. Tansverse plastronal fold forms acute angle; inframarginal scutes form groove; hatchling pigmentation and morphology present; specimen volume greater than yolk volume ratios 1.5 to 4:1. Stage 29 [86.0 ± 2 %DT]
28b. Not as above29
29a. Remaining yolk mass covered with pigmented membrane; inframarginal scutes folded near plastron; yolk mass less than one-half the volume of unpipped specimenStage 30 [94.7 ± 2 %DT]
29b. Embryo pipped with at least front flippers out of eggs shell30
30a. Embryo pipped; yolk mass mostly withdrawn into abdomen; transverse plastronal fold forms an acute angle; moist membranes still attached; specimen not ready to emergeStage 31a [100 ± 2 %DT]
30b. Embryo out of eggshell; yolk mass absent; transverse plastronal fold forms an oblique angle or nearly absent; any attached membranes appear abraded; specimen ready to emergeStage 31b [102 ± 2 %DT]
Although stages of development are discrete and separated by unambiguous changes in morphology, development is a continuous process, and specimens may exhibit characters intermediate between two stages. In these cases, adding a + to the stage number to indicate that the embryo exhibits a set of characteristics that is more advanced than the stage description helps to better define the position of the specimen in the developmental sequence (e.g., stage 16+ indicates a specimen that exhibits 26 pairs of somites but has only 2 pharyngeal clefts open). Where specific staging is required, the key should be used in conjunction with the detailed descriptions of Miller (1985b) to determine the stage of development.
The first group of postovipositional stages (6–10) was defined by changes in the shape of the blastopore and by differentiation of the notochord, neural folds, and head folds (Fig. 1). Stages 11–22 were defined by the number of somites, differentiation of the head, pigmentation of the eyes, and pharyngeal clefts. Later stages (23–31) were defined by carapace formation, development of pigmentation and scales, and the change in volume of the embryo relative to the volume of the yolk (Table 1).
Table 1.
Embryo volume and yolk volume relationships in late stage marine turtle embryos incubated at 29°C.
The interval between the mean times of stage 6 (oviposition) and stage 7 may exceed 18 hrs because eggs must equilibrate to the temperature of the sand and be released from their oviducal diapause (sensu preovipositional arrest; Rafferty and Reina 2012). For eggs incubated at 29°C, the mean times of stages 7 and 8 are separated by approximately 10 hrs. The mean intervals between stages 8 and 12 were short, being about 6–8 hrs each. One-day (24-hr) intervals occurred between stages 12 and 14. The mean interval increased to 1.5 d between stages 14 and 19; stages 19–24 were separated by intervals of 2 d. For stages 24–30, the mean interval between the mean times of the stages was slightly over 4 d (4.2 d). The sum of these intervals equaled 50 d of embryonic development. The interval between rupturing (pipping) and exiting the eggshell was between 1.5 and 5.6 d and varied with temperature (Table 2). Digging out of the nest chamber to emerge onto the beach surface varied with temperature (Table 3) and may involve an additional 1–7 or more days (Christens 1990; Godfrey and Mrosovsky 1997; Houghton and Hays 2001; Koch et al. 2008). In total, this schedule predicts that hatchlings should emerge onto the beach approximately 55 d (range, 51–59 d) following oviposition for eggs incubated at 29°C.
Table 2.
Elapsed days from first pipping to last hatching among eggs incubated at different temperatures (see also Christens 1990; Godfrey and Mrosovsky 1997; Houghton and Hays 2001; Koch et al. 2008). SD = standard deviation; df = degrees of freedom. NS = not significant.
Table 3.
Duration of incubation of eggs from 3 species of marine turtles at 3 different constant temperatures. Degree-days equals difference in mean days divided by difference in degrees.
The timing of the occurrence of a stage within the embryonic sequence depended on the temperature during development (Fig. 3; Table 3). At 26°C, the mean duration of incubation to emergence for the 3 species (77.9 d) was 23.2 d longer than at 29°C, which was 7.7 d longer than at 32°C. The duration of incubation was shortened by 2.6 d for each degree between 29°C and 32°C, whereas the duration was shortened by 7.7 d per degree between 26°C and 29°C.
Measurements of embryos (Tables 4–7) can be used to provide confirmation of the stage of development determined using the key. Total disc length (Table 4) is the first measureable characteristic exhibited by early stage embryos (stages 6–10). The mean total disc length of embryos of 4 species is about 0.2 cm. Crown-to-rump length (Table 4) became measurable as the head fold developed (stage 11) and continued to be useful through stage 20. The forelimb (Table 5) began to differentiate enough to be measured at stage 18; it continued to be useful as a confirmation of stage until stage 30, after which its length did not change. Straight carapace length (Table 6) became measurable during stage 23, when the posterior margin of the carapace was indicated; it was useful after the anterior margin of the carapace formed over the neck (stage 24) as a confirmation of stage until stage 28, after which its length did not change because of the embryonic curvature imposed by the eggshell.
Table 4.
Measurements of selected embryonic characteristics: total disc length (mm) and crown-to-rump length (mm). Stages from Miller (1985b); measurements from Miller (1982). Total disc length was measured as the straight distance between the anterior and posterior of the embryonic disc; crown-to-rump length was measured as the straight distance from the top head of the curled embryo to the curl at the base of the tail. SD = standard deviation.
Table 5.
Measurements of selected embryonic characteristics: forelimb length (mm). Stages from Miller (1985b); measurements from Miller (1982). Forelimb length was measured as the straight distance between the proximal and distal ends of the flipper manus of the developing embryo. SD = standard deviation.
Table 6.
Measurements of selected embryonic characteristics: straight carapace length (mm). Stages from Miller (1985b); measurements from Miller (1982). Straight carapace length was measured as the straight distance between the anterior and posterior ends of the carapace of the developing embryo. SD = standard deviation.
Table 7.
Selected measurements for later stage leatherback embryos of D. coriacea. Stages from Miller (1985b); measurements from Miller (1982). Straight carapace length was measured as the straight distance between the anterior and posterior ends of the carapace of the developing embryo. Straight carapace width was measured as the straight distance across the carapace of the developing embryo. Forelimb length was measured as the straight distance between the proximal and distal ends of the flipper manus of the developing embryo.
Measurements of flatback and green turtle embryos (Tables 4–6) can be used as a general proxy to help estimate the stage of young leatherback embryos during stages 6–22 because these embryos are larger than those of the other Cheloniide species. To assess older leatherback embryos (stages 23–31), the selected measurements shown in Table 7 can be used. Late stage embryos (stages 27–31) of all species can be staged by determining the ratio of the volume of the embryo (exclusive of yolk and membranes) to the yolk as the embryo progresses through these stages (Table 1).
DISCUSSION
Traditionally, a standard series of embryonic stages describes sequential morphological changes coordinated with the chronological age and size of the embryo incubated under defined conditions and provides illustrations of the embryonic stages (Yntema 1968; Mahmoud et al. 1973; Ewert 1985; Ferguson 1985; Miller 1985a, 1985b; Renous et al. 1989). Although the numbering and interval between stages, as well as the morphological characteristics that are described in a stage, vary somewhat among the several standard staging schemes for turtles, the selection of morphological characteristics used to define stages is not arbitrary (e.g., opening of pharyngeal clefts, formation of limbs, expression of scales, and pigmentation) because turtle embryos exhibit the same general suite of morphological characters in the same general sequence during development (Agassiz 1857; Yntema 1968; Mahmoud et al. 1973; Crastz 1982; Ewert 1985; Miller 1985b; Greenbaum 2002; Greenbaum and Carr 2002; Werneburg 2009).
All turtles oviposit their eggs during middle gastrulation (Ewert 1985; Werneburg 2009), and as a result, most staging tables for turtles begin at oviposition (e.g., stage 0 for Chelydra serpentina; Yntema 1968) even though development begins at fertilization in the oviduct. In contrast, the 5 preovipositional stages described for sea turtles (Miller 1985b) placed oviposition at stage 6; consequentially, we used stage 6 for oviposition in the key.
This key is based on the assumptions 1) that development of external morphological characters is similar among all species of marine turtles (Miller 1985b) and 2) that under the same conditions of incubation, the variation in the rate of development and the timing of the expression of morphological characteristics among embryos within eggs of the same clutch is small and the variation between clutches reduced (Miller 1985b). These assumptions are supported because throughout early and middle development, the embryos of all species of marine turtles are remarkably similar. As development progresses, clear differences between taxonomic groups appear at the following points: between the 2 families at stage 23 and among the genera at stage 25. Species characteristics become evident at stage 26, at which point adult identification keys can be used to identify species of embryos based on scalation (e.g., Bustard 1972; Pritchard and Mortimer 1999).
Following stage 27, the main embryonic changes involve growth (i.e., expressed as increased embryonic volume and corresponding decreased yolk volume) and the formation of the transverse plastronal fold caused by the bending of the embryo as it increases in size within the confines of the eggshell. Consequently, during the last ∼ 20% of the developmental period, staging relies on assessing the ratio of the volume of the embryo to that of the remaining yolk and the general angle displayed by the transverse plastronal fold. Crastz (1982) used embryonic volume as a measure of development and found that it had a reasonable correlation to days of development (R2 = 0.96). Stage 31a represents an embryo that has completed embryonic development and is in the process of extricating itself from the ruptured (pipped) eggshell. At stage 31b, the embryo has exited the eggshell, has begun to uncurl its body from the curved position it maintained inside the eggshell, and has withdrawn most of the remnant yolk into its abdomen; abraded extraembryonic membranes may still be attached.
The various species of marine turtles produce eggs of different sizes (i.e., diameter and mass) that, in turn, produce hatchlings of different sizes (Van Buskirk and Crowder 1994; Miller 1997). It follows that embryos of the various species will differ in size even though they express the same representative characteristics of a given embryonic stage. Even within a species, using a suite of morphological criteria to define a stage is more consistent than measurements (Yntema 1968). Therefore, measurements of specific characters (e.g., carapace length and crown-to-rump length) are not used to define a developmental stage in the key. However, measurements of embryos (Tables 4–7) can be used to provide confirmation of the stage of development determined using the key. Measurements of single characteristics are useful, but a combination of multiple characteristics provides better definition of the stage.
Because morphological changes occur rapidly at first and then more slowly as development proceeds, the initial stages span shorter time periods than the later stages. At 29°C, the sum of the time intervals between stages equals approximately 50 d from oviposition (stage 6) to pipping (stage 31a). Allowing for variation as a result of 1) temperature fluctuations during development, 2) the time required for pipping and leaving the eggshell, and 3) the time needed to dig out of the nest chamber, hatchlings are predicted to emerge onto the beach approximately 55 d following oviposition. Although incubation time varies among species and within a species at different locations (Hirth 1980; Van Buskirk and Crowder 1994; Limpus 2009), the 55-d schedule approximates the incubation time to emergence for most of the Cheloniidae (e.g., average 55.6 d and range 47–90 d in Queensland, Australia; Limpus 2009). In contrast, leatherback hatchlings, which typically emerge from deeper nests, usually require more time to reach the surface of the sand (approximately 60 d; Eckert et al. 2012).
In field studies, the “duration of incubation” is usually defined as the period from oviposition to the emergence of the hatchlings onto the beach surface (Márquez et al. 1976; Balazs 1980; Dodd 1988; Márquez 1994; Witzell 1983; Godfrey and Mrosovsky 1997; Hirth 1997; Limpus 2009; Eckert et al. 2012). In contrast, the “end of the embryonic period” occurs when the embryo pips and exits the eggshell (sensu Ewert 1979), which is several days prior to the emergence of the hatchlings onto the beach surface (Godfrey and Mrosovsky 1997). Temperature, as well as characteristics of the beach substrate, can modify the interval between hatching in the egg chamber and emergence onto the beach by several days (Table 2) (Christens 1990; Godfrey and Mrosovsky 1997; Houghton and Hays 2001; Koch et al. 2008). For this reason, rupturing of the eggshell (pipping) is a better measure of the end of incubation than is emergence from the nest (Gutzke et al. 1984). Taking into account reported interval variation, Godfrey and Mrosovsky (1997) suggested using 5 d as a reasonable estimate of the interval between pipping and emergence onto the beach, but this can vary between nesting sites and needs to be assessed on a site-by-site basis.
The key provided here addresses a need so that extrapolation from staging tables from nonmarine species and the associated problems can be avoided. Although many of the morphological criteria derived from nonmarine turtle species are applicable to marine turtle development, problems may occur when direct comparisons are attempted (Blanck and Sawyer 1981). Yntema and Mrosovsky (1982) applied Yntema's (1968) stages for C. serpentina successfully to C. caretta embryos. Determining the timing of developmental events, however, is difficult because staging tables for nonmarine turtle species have been based on embryos incubated (at least in part) at temperatures lower than those at which marine turtle eggs normally incubate (e.g., 20°C, C. serpentina, Yntema 1968; 21°C and 23°C, Chrysemys picta belli, Mahmoud et al. 1973).
In addition, as a result of the insulating effect of the substrate on the interactions among the hydric, gaseous, and temperature conditions experienced by the embryos, a delay of several hours or more may occur before changes in environmental conditions impact the embryos (Lolavar and Wyneken 2015). In the context of fluctuation in the environmental conditions of the beach, the variation in the prediction of developmental schedule is acceptable because these exogenous events do not have an instantaneous impact on the embryos.
A combination of determining hatching success (sensu Miller 1999) and assessing the stage of development of marine turtle embryos contained in eggs that did not hatch can contribute to an understanding of mortality factors operating on the nesting beach (Özdemir et al. 2008) or in a managed hatchery. Although retrieving a middle to late stage embryo is usually straight forward (albeit messy), autolysis of tissues in early stage embryos that died within the oviduct or within hours of oviposition (stages 2–10; Miller 1985b) can make it difficult to identify the presence of the embryo when a dead egg is opened some 2 mo later following the emergence of hatchlings from the nest (Wyneken et al. 1988). Therefore, the failure to find an embryo in such eggs does not necessarily equate to the egg not being fertilized.
When this simplified key to developmental stages is used in conjunction with knowledge of beach temperature and duration of incubation, it can aid estimation of when mortality occurred. In conjunction with review of data available for environmental parameters such as nest depth, position on the beach, tidal cycle, storm patterns, and rainfall, use of the key can help identify likely causes of mortality and can help with the design and assessment of field-based experiments.
Acknowledgments
We wish to acknowledge help of the members of the Queensland Turtle Research Project for their field assistance. Embryos were collected under permits held by C.J.L. Linda Bridges prepared the drawings.