Vanessa Conceição Coimbra’s research while affiliated with Federal University of Para and other places

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Publications (2)

Alternative protocol for the histological preparation of animal tissues
  • Article

March 2025

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12 Reads

Tissue and Cell

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Raquel dos Santos Braga

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Illustration depicting the experimental design, highlighting the collection time of Rhamdia quelen larvae from fresh and cryopreserved sperm. (T) treatment; (D.A.H) day(s) after hatching; (N) number of selected larvae
Sperm motility and kinetic parameters. A Sperm motility (p < 0.0001); B BCF (p < 0.0001); C VCL (p = 0.2767); D) VAP (p = 0.6701); E VSL (p = 0.9885); F STR (p = 0.0206); G WOB (p = 0.0531); H PROG (p = 0.0002). Significant difference by Student’s t test (*p < 0.05; *** p < 0.001; **** p < 0.0001). Mean ± SD. Fresh (n = 10), Cryopreserved (n = 8)
Evaluation of sperm morphology and pathologies. A Normal spermatozoa (p < 0.0001); B macrocephaly (%) (p < 0.0001); C microcephaly (%) (p < 0.0001); D loose head (%) (p < 0.0001); E degenerated head (%) (p < 0.0001); F proximal gout (%) (p = 0.2745); G distal gout (%) (p < 0.0001); H distal curled tail (%) (p = 0.0028); I strongly curled tail (%) (p < 0.0001); J broken tail (%) (p < 0.0001); K folded tail (%) (p = 0.0021); L short tail (%) (p < 0.0001). Significant difference by Mann–Whitney test (*p < 0.05; ** p < 0.01; *** p < 0.001; **** p < 0.0001). Graphs: Box and Whiskers = median, max, and min. n = 12
Results of the fertilization experiment with fresh and cryopreserved sperm. A Fertilization rate (p = 0.0163). B Hatching rate (p = 0.1748). Significant difference by Student’s T test (*p < 0.05). Mean ± SD. N = 12
Morphological characteristics of Silver catfish (Rhamdia quelen) larvae in six described stages of early development: A yolk larva, B pre-flexion, C early flexion, D flexion, E early post-flexion, F post-flexion. ov optic vesicle, n notochord, double arrow barbel pores, dashed arrow anal pore, y yolk, ef embryonic fin, dashed arrow anal pore, M mouth, b barbels, arrowhead anal rays, dt digestive tract, thick arrow dorsal complex, hollow arrow anal complex, asterisk dorsal rays. (n = 15 per treatment)

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Cryopreserved sperm does not affect larval ontogeny and quality in Rhamdia quelen
  • Article
  • Full-text available

February 2025

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35 Reads

Fish Physiology and Biochemistry

Vanessa Conceição Coimbra

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Raquel Santos dos Santos

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Fish sperm cryopreservation is an important technique for optimizing juvenile production in aquaculture stations and laboratories and contributing to the conservation of endangered species. Despite its benefits, the cryopreservation process can cause cellular damage, affecting spermatozoa quality and offspring viability. This study aimed to evaluate the larval development of jundiá Rhamdia quelen originating from cryopreserved sperm. Larvae were obtained from artificial reproduction using oocyte samples from four females combined with fresh (Control) or cryopreserved/thawed sperm. The semen was diluted in the cryoprotective solution (1:3 ratio) consisting of skimmed milk powder (5%), methanol (10%), and fructose (5%), and was packaged into 0.25 mL straws. The straws were then stored and cooled in liquid nitrogen vapor for 18 h. The straws were individually warmed in a water bath at 25 °C for 10 s to thaw the samples. The experiments were performed in triplicates. Sperm quality, fertilization, hatching, and larval development were evaluated. After larval hatching, six larval collections were performed (5, 10, 15, 20, and 25 days after hatching), and 15 larvae were sampled per collection per treatment. Cryopreservation reduced sperm motility (70.48 ± 7.70 fresh to 41.36 ± 4.80 cryopreserved semen), progressivity (3874 fresh to 2505 cryopreserved semen), and beat cross frequency (55.83 ± 155 fresh to 50.22 ± 190 cryopreserved semen). Increased the percentage of sperm with abnormal morphology and increased most sperm pathologies. Furthermore, the fertilization rate was lower in the cryopreserved group (63.1 ± 18, and 83.72 ± 7.59 for fresh semen), while hatching was not different between groups (65.3 ± 18.05 fresh, 48.89 ± 21.77 cryopreserved semen) Otherwise, the initial larval development morphology showed no difference in the appearance of structures such as the presence of the vitelline structure, pigmentation pattern, development of the anal pore, embryonic membrane, eye, barbells, notochord flexion, and fin rays, for both treatments. There was no significant difference in the frequency of structures between larvae from fresh and cryopreserved/thawed sperm, revealing a similar developmental pattern in both treatments. In conclusion, the cryopreservation protocol affects sperm quality; however, those sperm able to fertilize the oocytes originate normal larvae with regular larval development of R. quelen up to 25 days old. Graphical Abstract

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