The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳反应的接触脑脊液神经元的胞体及。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

要本文应用二叶酸(DHFA)和辅酶Ⅱ(NADPH)的质，建立了二叶酸还原酶(DHFR)活力测定的反应体系，并对酸度等反应条件进行了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳性反应的接触脑脊元的胞体及突起。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘要本文应用二(DHFA)和辅酶Ⅱ(NADPH)的荧光性质，建立了二还原酶(DHFR)活力测定的反应体系，并对度等反应条件进行了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳性反应接触脑脊液神经元胞体及突起。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘应用二叶酸(DHFA)和Ⅱ(NADPH)荧光性质，建立了二叶酸还原(DHFR)活力测定反应体系，并对酸度等反应条件进行了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳性反应的接触神经元的胞体及突起。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘要本文应用二叶(DHFA)和辅酶Ⅱ(NADPH)的荧光性质，建立了二叶酶(DHFR)活力测定的反应体系，并对度等反应条件进行了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳性反应的接触脑脊液神经元的胞体及突起。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘要本文应用二叶酸(DHFA)和辅酶Ⅱ(NADPH)的荧光性质，建立了二叶酸还原酶(DHFR)活力测定的反应体系，并对酸度等反应条件进行了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳性反应的接触脑脊液神经元的胞体及突起。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘要本文应用二叶酸(DHFA)和Ⅱ(NADPH)的荧光性质，建立了二叶酸还原(DHFR)活力测定的反应体系，并对酸度等反应条件了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

内可见呈阳性反应的接触脑脊液神经元的胞体及突起。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘要本文应用二叶(DHFA)和辅酶Ⅱ(NADPH)的荧光性质，建立了二叶还原酶(DHFR)活力测定的反应体系，并等反应条件进行了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳反应的接触脑脊液神经元的胞体。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘要本文应用二叶酸(DHFA)和辅酶Ⅱ(NADPH)的荧，建立了二叶酸还原酶(DHFR)活力测定的反应体系，并对酸度等反应条件进行了优化。

The perikaryon and process of the CSF contacting neurons in the periventricular nucleus were also in NADPH positive reaction.

室周核内可见呈阳性反的接触脑脊液神经元的胞体及突起。

A method for fluorophotometric assay of dihydrofolate reductasc (DHFR) activity by the use of fluorescence properties of dihydrofolate (DHFA) and NADPH was developed.

摘要本二叶(DHFA)酶Ⅱ(NADPH)的荧光性质，建立了二叶还原酶(DHFR)活力测定的反体系，并对度等反条件进行了优化。