Mm. Abbassy et al., EMBRYOGENESIS OF THE SAND FLY PHLEBOTOMUS-PAPATASI (DIPTERA, PSYCHODIDAE) - CELL CLEAVAGE, BLASTODERM FORMATION, AND GASTRULATION, Annals of the Entomological Society of America, 88(6), 1995, pp. 809-814
Serial sections of dechorionated eggs were used to study the early emb
ryology of the sand fly Phlebotomus paptasi (Scopoli) up to 96 h. Clea
vage began between oviposition and the first 12, h and continued until
the cellular blastoderm was formed (60 h). Cleavage was synchronous,
with most cleavage processes occurring during the first 36 h. Anterior
-to-posterior cellular growth became apparent until division temporari
ly ceased. Cleavage nuclei were observed Ist in the anterior 1/3 of th
e egg and, as they developed, became more evenly distributed into the
periplasm. Primary vitellophages concentrated linearly in the center o
f the egg started migrating posteriorly, and a few secondary vitelloph
ages appeared at the posterior pole. Approximately 6-10 pole cells ori
ginated from the blastoderm and were formed at the posterior extremity
. At 48 h, delimiting cell furrows first became evident, jutting inwar
d from the outer periplasmic membrane between the nuclei, and continue
d until 60 h. Invagination of the germ band occurred 72 h after ovipos
ition and spread bilaterally as paired ventrolateral mesodermal bands.
The stomodeum and the anterior midgut invaginated simultaneously at 7
2-84 h. Formation and invagination of stomodeal cells preceded that of
the proctodeum. The proctodeal invagination began at 84 h, enclosing
the pole cells, which migrated from the posterior pole to the dorsal s
ide of the egg. Invagination of the pole cells appeared in association
with the invaginating posterior midgut proctodeal complex. The amnion
and serosa became a loosely attached layer of cells clumped to form a
primary dorsal organ, which underwent lysis at 84 h and was totally r
esorbed into the yolk by 96 h.