Refrigeration Medium – TYB with Gentamicin

Here are the density and density gradients of ISolate.

To obtain a 40% upper layer from our 50% ISolate Upper Layer, mix 8.0 mL of (upper layer) with 2.0 mL of Modified HTF Medium with Gentamicin - HEPES.

To obtain an 80% lower layer from our 90% ISolate Lower Layer, mix 8.9 mL of lower layer with 1.1 mL of Modified HTF Medium with Gentamicin - HEPES.

We recommend using prepared ISolate gradient within two hours of preparation to avoid the mixing of the gradient prior to use.

ISolate uses a density gradient centrifugation technique as the method of separation. The gradients increase in density from the top to the bottom of the preparation, the sample is gently placed on top of the preparation, and centrifuged. During the process highly motile sperm cells actively move in the direction of the sedimentation gradient. This is in contrast to poorly motile/ immotile sperm cells that do not penetrate the boundaries of the gradient. Upon completion of the centrifugation highly motile sperm cells are enriched in a pellet at the bottom of the preparation¹.

References

1. Henkel, R. R., & Schill, W. B. (2003). Sperm preparation for ART. Reprod Biol Endocrinol. Nov;14;1:108.
2. Hammadeh, M.E., Greiner, P., Rosenbaum, P., Schmidt, W. (2001). Comparison Between Human Sperm Preservation Medium and TEST-Yolk Buffer on Protecting Chromatin and Morphology Integrity of Human Spermatozoa in Fertile and Subfertile Men After Freeze-Thawing Procedure. J Androl. Nov-Dec;22(6):1012-8.
3. Wolf, D. P., Patton, P. E., Burry, K. A., & Kaplan, P. F. (2001). Intrauterine insemination–ready versus conventional semen cryopreservation for donor insemination: a comparison of retrospective results and a prospective, randomized trial. Fertil Steril. Jul;76(1):181-5.
4. Larson, J. M., McKinney, K. A., Mixon, B. A., Burry, K. A., & Wolf, D. P. (1997). An intrauterine insemination-ready cryopreservation method compared with sperm recovery after conventional freezing and post-thaw processing*. Fertil Steril. July; 68(1), 143–148.
5. Medranoa L., Encisob M., Gomez-Torresc M.J., Aizpuruaa J. (2019). First birth of a healthy infant following intra-cytoplasmic sperm injection using a new permeable cryoprotectant-free sperm vitrification protocol. Cryobiology, 2019 Apr;87:117-119.
6. Optimization of sperm culture conditions for human ART. Charles L. Bormann and Carol L. Curchoe.

The addition of antibiotics to sperm washing media is at the discretion of the end user. Please reference your own clinic’s protocols when adding antibiotics. For additional details, each laboratory should consult its own laboratory procedures and protocols which have been specifically developed and optimized for your individual medical program. Please reference table below for a complete list of sperm processing products and gentamicin content.

Nexpring Health recommends the following protocol for thawing raw semen and processed sperm.

Yes, ISolate can be diluted with Sperm Washing Medium, or with Modified HTF Medium with Gentamicin - HEPES.

This table details the cryoprotectant, intended use, and use ratio of our sperm preparation media.

^† Capacitation at room temperature for approximately two hours.

These are the storage instructions for UNOPENED items.

Here is the shelf life for OPENED items.

No, Refrigeration Medium - TYB is intended for short term refrigerated sperm storage. Refrigeration Medium- TYB is typically used to store sperm for up to 96 hours between 2-8°C, transporting semen, and as an aid in sperm capacitation for conventional fertilization.

For freezing sperm we recommend using Freezing Medium - TYB with Glycerol & Gentamicin or Arctic Sperm Cryopreservation Medium.

Both products are intended to be single use and we recommend discarding any excess medium that remains after the procedures are completed. To optimize usage of your product, we recommend thawing the bottle/vial and aseptically aliquoting the media into smaller sterile bottles/vials and stored as directed on the product insert. Do not use aliquots that show a shift in color, particulate matter or any evidence of contamination.

This product is for customers who prefer to freeze sperm without the use of test yolk buffer for long term storage. The product should be used in a ratio of 3:1 (sperm:Arctic).

In general, the recovery rate is around 50% post-thaw when using Freezing Medium - TYB with Glycerol & Gentamicin.

We recommend that the TYB freezing medium should be removed prior to IUI either by simple washing with Sperm Washing Medium or Multipurpose Handling Medium - Complete, or if washing thawed raw semen, by density gradient centrifugation with ISolate²,³,⁴.

References

1. Henkel, R. R., & Schill, W. B. (2003). Sperm preparation for ART. Reprod Biol Endocrinol. Nov;14;1:108.
2. Hammadeh, M.E., Greiner, P., Rosenbaum, P., Schmidt, W. (2001). Comparison Between Human Sperm Preservation Medium and TEST-Yolk Buffer on Protecting Chromatin and Morphology Integrity of Human Spermatozoa in Fertile and Subfertile Men After Freeze-Thawing Procedure. J Androl. Nov-Dec;22(6):1012-8.
3. Wolf, D. P., Patton, P. E., Burry, K. A., & Kaplan, P. F. (2001). Intrauterine insemination–ready versus conventional semen cryopreservation for donor insemination: a comparison of retrospective results and a prospective, randomized trial. Fertil Steril. Jul;76(1):181-5.
4. Larson, J. M., McKinney, K. A., Mixon, B. A., Burry, K. A., & Wolf, D. P. (1997). An intrauterine insemination-ready cryopreservation method compared with sperm recovery after conventional freezing and post-thaw processing*. Fertil Steril. July; 68(1), 143–148.
5. Medranoa L., Encisob M., Gomez-Torresc M.J., Aizpuruaa J. (2019). First birth of a healthy infant following intra-cytoplasmic sperm injection using a new permeable cryoprotectant-free sperm vitrification protocol. Cryobiology, 2019 Apr;87:117-119.
6. Optimization of sperm culture conditions for human ART. Charles L. Bormann and Carol L. Curchoe.

Nexpring Health has not performed studies to confirm this usage and does not recommend the combined usage of its reagents with those from other vendors. However, independent recent studies report usage of MHM-C with other vitrification reagents and protocols⁵.

References

1. Henkel, R. R., & Schill, W. B. (2003). Sperm preparation for ART. Reprod Biol Endocrinol. Nov;14;1:108.
2. Hammadeh, M.E., Greiner, P., Rosenbaum, P., Schmidt, W. (2001). Comparison Between Human Sperm Preservation Medium and TEST-Yolk Buffer on Protecting Chromatin and Morphology Integrity of Human Spermatozoa in Fertile and Subfertile Men After Freeze-Thawing Procedure. J Androl. Nov-Dec;22(6):1012-8.
3. Wolf, D. P., Patton, P. E., Burry, K. A., & Kaplan, P. F. (2001). Intrauterine insemination–ready versus conventional semen cryopreservation for donor insemination: a comparison of retrospective results and a prospective, randomized trial. Fertil Steril. Jul;76(1):181-5.
4. Larson, J. M., McKinney, K. A., Mixon, B. A., Burry, K. A., & Wolf, D. P. (1997). An intrauterine insemination-ready cryopreservation method compared with sperm recovery after conventional freezing and post-thaw processing*. Fertil Steril. July; 68(1), 143–148.
5. Medranoa L., Encisob M., Gomez-Torresc M.J., Aizpuruaa J. (2019). First birth of a healthy infant following intra-cytoplasmic sperm injection using a new permeable cryoprotectant-free sperm vitrification protocol. Cryobiology, 2019 Apr;87:117-119.
6. Optimization of sperm culture conditions for human ART. Charles L. Bormann and Carol L. Curchoe.

A study by Bormann and Curchoe demonstrated the superior performance of dual-buffer solution of HEPES and MOPS containing Multipurpose Handling Medium - Complete (MHM-C) for key sperm parameters over single buffer controls⁶.

References

1. Henkel, R. R., & Schill, W. B. (2003). Sperm preparation for ART. Reprod Biol Endocrinol. Nov;14;1:108.
2. Hammadeh, M.E., Greiner, P., Rosenbaum, P., Schmidt, W. (2001). Comparison Between Human Sperm Preservation Medium and TEST-Yolk Buffer on Protecting Chromatin and Morphology Integrity of Human Spermatozoa in Fertile and Subfertile Men After Freeze-Thawing Procedure. J Androl. Nov-Dec;22(6):1012-8.
3. Wolf, D. P., Patton, P. E., Burry, K. A., & Kaplan, P. F. (2001). Intrauterine insemination–ready versus conventional semen cryopreservation for donor insemination: a comparison of retrospective results and a prospective, randomized trial. Fertil Steril. Jul;76(1):181-5.
4. Larson, J. M., McKinney, K. A., Mixon, B. A., Burry, K. A., & Wolf, D. P. (1997). An intrauterine insemination-ready cryopreservation method compared with sperm recovery after conventional freezing and post-thaw processing*. Fertil Steril. July; 68(1), 143–148.
5. Medranoa L., Encisob M., Gomez-Torresc M.J., Aizpuruaa J. (2019). First birth of a healthy infant following intra-cytoplasmic sperm injection using a new permeable cryoprotectant-free sperm vitrification protocol. Cryobiology, 2019 Apr;87:117-119.
6. Optimization of sperm culture conditions for human ART. Charles L. Bormann and Carol L. Curchoe.

Components of cryopreservation media are different for sperms and oocytes/embryos. FUJIFILM Irvine Scientific offers specific media for this application. Please consider Vit Kit-Freeze and Vit Kit-Thaw for oocytes and embryos.